Engineered CRISPR-Cas9 nucleases

ABSTRACT

Engineered CRISPR-Cas9 nucleases with improved specificity and their use in genomic engineering, epigenomic engineering, genome targeting, and genome editing.

CLAIM OF PRIORITY

This application claims priority under 35 USC § 119(e) to U.S. Patent Application Ser. Nos. 62/211,553, filed on Aug. 28, 2015; 62/216,033, filed on Sep. 9, 2015; 62/258,280, filed on Nov. 20, 2015; and 62/271,938, filed on Dec. 28, 2015; and is a continuation in part of U.S. patent application Ser. No. 15/015,947, filed on Feb. 4, 2016, which claims the benefit of U.S. Patent Application Ser. Nos. 62/211,553, filed on Aug. 28, 2015; 62/216,033, filed on Sep. 9, 2015; and 62/258,280, filed on Nov. 20, 2015. The entire contents of the foregoing are hereby incorporated by reference.

FEDERALLY SPONSORED RESEARCH OR DEVELOPMENT

This invention was made with Government support under Grant Nos. DP1 GM105378 and R01 GM088040 awarded by the National Institutes of Health. The Government has certain rights in the invention.

SEQUENCE LISTING

The instant application contains a Sequence Listing which has been submitted electronically in ASCII format and is hereby incorporated by reference in its entirety. Said ASCII copy, created on Aug. 26, 2016, is named SEQUENCE LISTING.txt and is 129,955 bytes in size.

TECHNICAL FIELD

The invention relates, at least in part, to engineered Clustered Regularly Interspaced Short Palindromic Repeats (CRISPRs)/CRISPR-associated protein 9 (Cas9) nucleases with altered and improved target specificity and their use in genomic engineering, epigenomic engineering, genome targeting, genome editing, and in vitro diagnostics.

BACKGROUND

CRISPR-Cas9 nucleases enable efficient genome editing in a wide variety of organisms and cell types (Sander & Joung, Nat Biotechnol 32, 347-355 (2014); Hsu et al., Cell 157, 1262-1278 (2014); Doudna & Charpentier, Science 346, 1258096 (2014); Barrangou & May, Expert Opin Biol Ther 15, 311-314 (2015)). Target site recognition by Cas9 is programmed by a chimeric single guide RNA (sgRNA) that encodes a sequence complementary to a target protospacer (Jinek et al., Science 337, 816-821 (2012)), but also requires recognition of a short neighboring PAM (Mojica et al., Microbiology 155, 733-740 (2009); Shah et al., RNA Biol 10, 891-899 (2013); Jiang et al., Nat Biotechnol 31, 233-239 (2013); Jinek et al., Science 337, 816-821 (2012); Sternberg et al., Nature 507, 62-67 (2014)).

SUMMARY

As described herein, Cas9 Proteins can be engineered to show increased specificity, theoretically by reducing the binding affinity of Cas9 for DNA. Thus, described herein are a number of Cas9 variants that have increased specificity (i.e., induce substantially fewer off target effects at imperfectly matched or mismatched. DNA sites) as compared to the wild type protein, as well as methods of using them.

In a first aspect, the invention provides isolated Streptococcus pyogenes Cas9 (SpCas9) proteins with mutations at one, two, three, four, five, six or all seven of the following positions: L169A, Y450, N497, R661, Q695, Q926, and/or D1135E e.g., comprising a sequence that is at least 80% identical to the amino acid sequence of SEQ ID NO:1 with mutations at one, two, three, four, five, six, or seven of the following positions: L169, Y450, N497, R661, Q695, Q926, D1135E, and optionally one or more of a nuclear localization sequence, cell penetrating peptide sequence, and/or affinity tag. A mutation alters the amino acid to an amino acid other than the native amino acid (e.g., 497 is anything but N). In preferred embodiments the mutation changes the amino acid to any amino acid other than the native one, arginine or lysine; in some embodiments, the amino acid is alanine.

In some embodiments, the variant SpCas9 proteins comprise mutations at one, two, three, or all four of the following: N497, R661, Q695, and Q926, e.g., one, two, three, or all four of the following mutations: N497A, R661A, Q695A, and Q926A.

In some embodiments, the variant SpCas9 proteins comprise mutations at Q695 and/or Q926, and optionally one, two, three, four or all five of L169, Y450, N497, R661 and D1135E, e.g., including but not limited to Y450A/Q695A, L169A/Q695A, Q695A/Q926A, Q695A/D1135E, Q926A/D1135E, Y450A/D1135E, L169A/Y450A/Q695A, L169A/Q695A/Q926A, Y450A/Q695A/Q926A, R661A/Q695A/Q926A, N497A/Q695A/Q926A, Y450A/Q695A/D1135E, Y450A/Q926A/D1135E, Q695A/Q926A/D1135E, L169A/Y450A/Q695A/Q926A, L169A/R661A/Q695A/Q926A,Y450A/R661A/Q695A/Q926A, N497A/Q695A/Q926A/D1135E, R661A/Q695A/Q926A/D1135E, and Y450A/Q695A/Q926A/D1135E.

In some embodiments, the variant SpCas9 proteins comprise mutations at N14; S15; S55; R63; R78;H160; K163; R165; L169; R403; N407; Y450; M495; N497; K510; Y515; W659; R661; M694; Q695; H698; A728; S730;1K775; S777; R778; R780; K782; R783; K789; K797; Q805; N808; K810; R832; Q844; S845; K848; S851; K855; R859; K862; K890; Q920; Q926; K961; S964; K968; K974; R976; N980; H982; K1003; K1014; S1040; N1041; N1044; K1047; K1059; R1060; K1107; E1108; S1109; K1113; R1114; S1116; K1118; D1135; S1136; K1153; K1155; K1158; K1200; Q1221; H1241; Q1254; Q1256; K1289; K1296; K1297; R1298; K1300; H1311; K1325; K1334; T1337 and/or S1216.

In some embodiments, the variant SpCas9 proteins also comprise one or more of the following mutations: N14A; S15A; S55A; R63A; R78A; R165A; R403A; N407A; N497A; Y450A; K510A; Y515A; R661A; Q695A; S730A; K775A; S777A; R778A; R780A; K782A; R783A; K789A; K797A; Q805A; N808A; K810A; R832A; Q844A; S845A; K848A; S851A; K855A; R859A; K862A; K890A; Q920A; Q926A; K961A; S964A; K968A; K974A; R976A; N980A; H982A; K1003A; K1014A; S1040A; N1041A; N1044A; K1047A; K1059A; R1060A; K1107A; E1108A; S1109A; K1113A; R1114A; S1116A; K1118A; D1135A; S1136A; K1153A; K1155A; K1158A; K1200A; Q1221A; H1241A; Q1254A; Q1256A; K1289A; K1296A; K1297A; R1298A; K1300A; H1311A; K1325A; K1334A; T1337A and/or S1216A. In some embodiments, the variant proteins include HF1(N497A/R661A/Q695A/Q926A)+K810A, HF1+K848A, HF1+K855A, HF1-411982A, HF1+K848A/K1003A, HF1+K.848A/R1060A, 11F1+111(855A/K1003A, HF1+K855A/R1060A, HF1+H982A/K1003A, HF1+H982A/R1060A, HF1+K1003A/R1060A, HF1+K810A/K1003A/R1060A, HF1+K848A/K1003A/R1060A. In some embodiments, the variant proteins include HF1+K848A/K1003A, HF1+K848A/R1060A, HF1+K855A/K1003A, HF1+K855A/R1060A, HF1+K1003A/R1060A, HF1+K848A/K1003A/R1060A. In some embodiments, the variant proteins include Q695A/Q926A/R780A, Q695A/Q926A/R976A, Q695A/Q926A/H982A, Q695A/Q926A/K855A, Q695A/Q926A/K848A/K1003A, Q695A/Q926A/K848A/K855A, Q695A/Q926A/K848A/H982A, Q695A/Q926A/K1003A/R1060A, Q695A/Q926A/K848A/R1060A, Q695A/Q926A/K855A/H982A, Q695A/Q926A/K855A/K1003A, Q695A/Q926A/K855A/R1060A, Q695A/Q926A/H982A/K1003A, Q695A/Q926A/H982A/R1060A, Q695A/Q926A/K 1003A/R1060A, Q695A/Q926A/K810A/K1003A/R1060A, Q695A/Q926A/K 848A/K 1003A/R1060A. In some embodiments, the variants include N497A/R661A/Q695A/Q926A/K810A, N497A/R661A/Q695A/Q926A/K848A, N497A/R661A/Q695A/Q926A/K855A, N497A/R661A/Q695A/Q926A/R780A, N497A/R661A/Q695A/Q926A/K968A, N497A/R661A/Q695A/Q926A/H982A, N497A/R661A/Q695A/Q926A/K1003A, N497A/R661A/Q695A/Q926A/K1014A, N497A/R661A/Q695A/Q926A/K1047A, N497A/R661A/Q695A/Q926A/R1060A, N497AIR661A/Q695A/Q926A/K810A/K968A, N497A/R661A/Q695A/Q926A/K810A/K848A, N497A/R661A/Q695A/Q926A/K810A/K1003A, N497A/R661A/Q695A/Q926A/K810A/R1060A, N497A/R661A/Q695A/Q926A/K848A/K 1003A, N497A/R661A/Q695A/Q926A/K848A/R1060A, N497A/R661A/Q695A/Q926A/K855A/K1003A, N497A/R661A/Q695A/Q926A/K855A/R1060A, N497A/R661A/Q695A/Q926A/K968A/K1003A, N497A/R661A/Q695A/Q926A/H982A/K1003A, N497A/R661A/Q695A/Q926A/H982A/R1060A, N497A/R661A/Q695A/Q926A/K1003A/R1060A, N497A/R661A/Q695A/Q926A/K810A/K1003A/R1060A, N497A/R661A/Q695A/Q926A/K848A/K1003A/R1060A, Q695A/Q926A/R780A, Q695A/Q926A/K810A, Q695A/Q926A/R832A, Q695A/Q926A/K848A, Q695A/Q926A/K855A, Q695A/Q926A/K968A, Q695A/Q926A/R976A, Q695A/Q926A/H982A, Q695A/Q926A/K1003A, Q695A/Q926A/K1014A, Q695A/Q926A/K1047A, Q695A/Q926A/R1060A, Q695A/Q926A/K848A/K968A, Q695A/Q926A/R976A, Q695A/Q926A/H982A, Q695A/Q926A/K855A, Q695A/Q926A/K848A/K1003A, Q695A/Q926A/K848A/K855A, Q695A/Q926A/K848A/H982A, Q695A/Q926A/K1003A/R1060A, Q695A/Q926A/R832A/R1060A, Q695A/Q926A/K968A/K1003A, Q695A/Q926A/K968A/R1060A, Q695A/Q926A/K848A/R1060A, Q695A/Q926A/K855A/H982A, Q695A/Q926A/K855A/K1003A, Q695A/Q926A/K855A/R1060A, Q695A/Q926A/H982A/K1003A, Q695A/Q926A/H982A/R 1060A, Q695A/Q926A/K1003A/R1060A, Q695A/Q926A/K810A/K1003A/R1060A, Q695A/Q926A/K1003A/K1047A/R1060A, Q695A/Q926A/K968A/K1003A/R1060A, Q695A/Q926A/R832A/K1003A/R1060A, or Q695A/Q926A/K848A/K1003A/R1060A.

Mutations to amino acids other than alanine are also included, and can be made and used in the present methods and compositions.

In some embodiments, variant SpCas9 proteins comprise one or more of the following additional mutations: R63A, R66A, R69A, R70A, R71A, Y72A, R74A, R75A, K76A, N77A, R78A, R115A, H160A, K163A, R165A, L169A, R403A, T404A, F405A, N407A, R447A, N497A, 1448A, Y450A, S460A, N1495A, K510A, Y515A, R661A, M694A, Q695A, H698A, Y1013A, V1015A, R1122A, K1123A, K1124A, K1158A, K1185A, K1200A, S1216A, Q1221A, K1289A, R1298A, K1300A, K1325A, R1333A, K1334A, R1335A, and T1337A.

In some embodiments, the variant SpCas9 proteins comprise multiple substitution mutations: N497/R661/Q695/Q926 (quadruple variant mutants); Q695/Q926 (double mutant); R661/Q695/Q926 and N497/Q695/Q926 (triple mutants). In some embodiments, additional substitution mutations at L169, Y450 and/or D1135 might be added to these double-, triple, and quadruple mutants or added to single mutants bearing substitutions at Q695 or Q926. In some embodiments, the mutants have alanine in place of the wild type amino acid. In some embodiments, the mutants have any amino acid other than arginine or lysine (or the native amino acid).

In some embodiments, the variant SpCas9 proteins also comprise one or more mutations that decrease nuclease activity selected from the group consisting of mutations at D10, E762, D839, H983, or D986; and at H840 or N863. In some embodiments, the mutations are: (i) D10A or D10N, and (ii) H840A, H840N, or H840Y.

In some embodiments, the SpCas9 variants can also include one of the following sets of mutations: D1135V/R1335Q/T1337R (VQR variant); D1135E/R1335Q/T1337R (EQR variant); D1135V/G1218R/R1335Q/T1337R (VRQR variant); or D1135V/G1218R/R1335E/T1337R (VRER variant).

Also provided herein are isolated Staphylococcus aureus Cas9 (SaCas9) protein, with mutations at one, two, three, four, five, six, or more of the following positions: Y211, Y212, W229, Y230, R245, T392, N419, Y651, or R654, e.g., comprising a sequence that is at least 80% identical to the amino acid sequence of SEQ ID NO:2 with mutations at one, two, three, four, or five, or six of the following positions: Y211, Y212, W229, Y230, R245, T392, N419, Y651, or R654, and optionally one or more of a nuclear localization sequence, cell penetrating peptide sequence, and/or affinity tag. In some embodiments, the SaCas9 variants described herein include the amino acid sequence of SEQ ID NO:2, with mutations at one, two, three, four, five, six, or more of the following positions: Y211, Y212, W229, Y230, R245, T392, N419, Y651 and/or R654. In some embodiments the variants include one or more of the following mutations: Y211A, Y212A, W229, Y230A, R245A, T392A, N419A, Y651, and/or R654A.

In some embodiments, the variant SaCas9 proteins comprise mutations at N419 and/or R654, and optionally one, two, three, four or more of the additional mutations Y211, Y212, W229, Y230, R245 and T392, preferably N419A/R654A, Y211A/R654A, Y211A/Y212A, Y211A/Y230A, Y211A/R245A, Y212A/Y230A, Y212A/R245A, Y230A/R245A, W229A/R654A, Y211A/Y212A/Y230A, Y211A/Y212A/R245A, Y211A/Y212A/Y651A, Y211A/Y230A/R245A, Y211A/Y230A/Y651A, Y211A/R245A/Y651A, Y211A/R245A/R654A, Y211A/R245A/N419A, Y211A/N419A/R654A, Y212A/Y230A/R245A, Y212A/Y230A/Y651A, Y212A/R245A/Y651A, Y230A/R245A/Y651A, R245A/N419A/R654A, T392A/N419A/R654A, R245A/T392A/N419A/R654A, Y211A/R245A/N419A/R654A, W229A/R245A/N419A/R654A, Y211A/R245A/T392A/N419A/R654A, or Y211A/W229A/R245A/N419A/R654A.

In some embodiments, the variant SaCas9 proteins comprise mutations at Y211; Y212; W229; Y230; R245; T392; N419; L446; Q488; N492; Q495; R497; N498; R499; Q500; K518; K523; K525; H557; R561; K572; R634; Y651; R654; G655; N658; S662; N667; R686; K692; R694; H700; K751; D786; T787; Y789; T882; K886; N888; 889; L909; N985; N986; R991; R1015; N44; R45; R51; R55; R59; R60; R116; R165; N169; R208; R209; Y211; T238; Y239; K248; Y256; R314; N394; Q414; K57; R61; H111; K114; V164; R165; L788; S790; R792; N804; Y868; K870; K878; K879; K881; Y897; R901; and/or K906.

In some embodiments, the variant SaCas9 proteins comprise one or more of the following mutations: Y211A; Y212A; W229A; Y230A; R245A; T392A; N419A; L446A; Q488A; N492A; Q495A; R497A; N498A; R499A; Q500A; K518A; K523A; K525A; H557A; R561A; K572A; R634A; Y651A; R654A; G655A; N658A; S662A; N667A; R686A; K692A; R694A; H700A; K751A; D786A; T787A; Y789A; T882A; K886A; N888A; A889A; L909A; N985A; N986A; R991A; R1015A; N44A; R45A; R51A; R55A; R59A; R60A; R116A; R165A; N169A; R208A; R209A; T238A; Y239A; K248A; Y256A; R314A; N394A; Q414A; K57A; R61A; H111A; K114A; V164A; R165A; L788A; S790A; R792A; N804A; Y868A; K870A; K878A; K879A; K881A; Y897A; R901A; K906A.

In some embodiments, variant SaCas9 proteins comprise one or more of the following additional mutations: Y211A, W229A, Y230A, R245A, T392A, N419A, L446A, Y651A, R654A, D786A, T787A, Y789A, T882A, K886A, N888A, A889A, L909A, N985A, N986A, R991A, R1015A, N44A, R45A, R51A, R55A, R59A, R60A, R116A, R165A, N169A, R208A, R209A, T238A, Y239A, K248A, Y256A, R314A, N394A, Q414A, K57A, R61A, H111A, K114A, V164A, R165A, L,788A, S790A, R792A, N804A, Y868A, K870A, K878A, K879A, K881A, Y897A, R901A, K906A.

In some embodiments, the variant SaCas9 proteins comprise multiple substitution mutations: R245/T392/N419/R654 and Y221/R245/N419/R654 (quadruple variant mutants); N419/R654, R245/R654, Y221/R654, and Y221/N419 (double mutants); R245/N419/R654, Y211/N419/R654, and T392/N419/R654 (triple mutants). In some embodiments the mutants contain alanine in place of the wild type amino acid.

In some embodiments, the variant SaCas9 proteins also comprise one or more mutations that decrease nuclease activity selected from the group consisting of mutations at D10, E477, D556, H701, or D704; and at H557 or N580. In some embodiments, the mutations are: (i) D10A or D10N, (ii) H557A, H557N, or H557Y (iii) N580A, and/or (iv) D556A.

In some embodiments, the variant SaCas9 proteins comprise one or more of the following mutations: E782K, K929R, N968K, or R1015H. Specifically, E782K/N968K/R1015H (KKH variant); E782K/K,929R/R 1015H (KRH variant): or E782K/K929R/N968K/R1015H (KRKH variant).

In some embodiments, the variant Cas9 proteins include mutations to one or more of the following regions to increase specificity:

Functional Region SpCas9 SaCas9 Residues contacting L169; Y450; M495; N497: Y211; W229; Y230; the DNA of the W659; R661; M694; Q695; R245; T392; N419; spacer region H698; A728; Q926; E1108; L446; Y651; R654 V1015 Residues that N14; S15; S55; S730; K775; Q488A; N492A; Q495A; potentially contact S777; R778; R780; K782; R783; R497A; N498A; R499; the DNA of the non- K789; K797; Q805; N808; Q500; K518; K523; target strand K810; R832; Q844; S845; K848; K525; H557; R561; S851; K855; R859; K862; K890; K572; R634; R654; Q920; K961; S964; K968; K974; G655; N658; S662; R976; N980; H982; K1003; N667; R686; K692; K1014; S1040; N1041; N1044; R694; H700; K751 K1047; K1059; R1060; K1200; H1241; Q1254; Q1256; K1289; K1296; K1297; K1300; H1311; K1325 Residues contacting R71; Y72; R78; R165; R403; D786; T787; Y789; the DNA of the PAM T404; F405; K1107; S1109; T882; K886; N888; region (including R1114; S1116; K1118; D1135; A889; L909; N985; direct PAM contacts) S1136; K1200; S1216; E1219; N986; R991; R1015 R1333; R1335; T1337 Residues contacting Y72; R75; K76; L101; S104; N44; R45; R51; R55; the RNA of the F105; R115; H116; I135; H160; R59; R60; R116; R165; spacer region K163; Y325; H328; R340; F351; N169; R208; R209; D364; Q402; R403; I1110; Y211; T238; Y239; K1113; R1122; Y1131 K248; Y256; R314; N394; Q414 Residues contacting R63; R66; R70; R71; R74; R78; K57; R61; H111; the RNA of the R403; T404; N407; R447; I448; K114; V164; R165; repeat/anti-repeat Y450; K510; Y515; R661; L788; S790; R792; region V1009; Y1013 N804; Y868; K870; K878; K879; K881; Y897; R901; K906 Residues contacting K30; K33; N46; R40; K44; E57; R47; K50; R54; R58; the RNA stem loops T62; R69; N77; L455; S460; H62; R209; E213; R467; T472; I473; H721; K742; S219; R452; K459; K1097; V1100; T1102; F1105; R774; N780; R781; K1123; K1124; E1225; Q1272; L783 H1349; S1351; Y1356

Also provided herein are fusion proteins comprising the isolated variant Cas9 proteins described herein fused to a heterologous functional domain, with an optional intervening linker, wherein the linker does not interfere with activity of the fusion protein. In some embodiments, the heterologous functional domain acts on DNA or protein, e.g., on chromatin. In some embodiments, the heterologous functional domain is a transcriptional activation domain. In some embodiments, the transcriptional activation domain is from VP64 or NF-κB p65. In some embodiments, the heterologous functional domain is a transcriptional silencer or transcriptional repression domain. In some embodiments, the transcriptional repression domain is a Kruppel-associated box (KRAB) domain, ERF repressor domain (ERD), or mSin3A interaction domain (SID). In some embodiments, the transcriptional silencer is Heterochromatin Protein 1 (HP1), e.g., HP1α or HP1β. In some embodiments, the heterologous functional domain is an enzyme that modifies the methylation state of DNA. In some embodiments, the enzyme that modifies the methylation state of DNA is a DNA methyltransferase (DNMT) or the entirety or the dioxygenase domain of a TET protein, e.g., a catalytic module comprising the cysteine-rich extension and the 2OGFeDO domain encoded by 7 highly conserved exons, e.g., the Tet1 catalytic domain comprising amino acids 1580-2052, Tet2 comprising amino acids 1290-1905 and Tet3 comprising amino acids 966-1678. In some embodiments, the TET protein or TET-derived dioxygenase domain is from TET1. In some embodiments, the heterologous functional domain is an enzyme that modifies a histone subunit. In some embodiments, the enzyme that modifies a histone subunit is a histone acetyltransferase (HAT), histone deacetylase (HDAC), histone methyltransferase (HMT), or histone demethylase. In some embodiments, the heterologous functional domain is a biological tether. In some embodiments, the biological tether is MS2, Csy4 or lambda N protein. In some embodiments, the heterologous functional domain is FokI.

Also provided herein are nucleic acids, isolated nucleic acids encoding the variant Cas9 proteins described herein, as well as vectors comprising the isolated nucleic acids, optionally operably linked to one or more regulatory domains for expressing the variant Cas9 proteins described herein. Also provided herein are host cells, e.g., bacterial, yeast, insect, or mammalian host cells or transgenic animals (e.g., mice), comprising the nucleic acids described herein, and optionally expressing the variant Cas9 proteins described herein.

Also provided herein are isolated nucleic acids encoding the Cas9variants, as well as vectors comprising the isolated nucleic acids, optionally operably linked to one or more regulatory domains for expressing the variants, and host cells, e.g., mammalian host cells, comprising the nucleic acids, and optionally expressing the variant proteins.

Also provided herein are methods of altering the genome or epigenome of a cell, by expressing in the cell or contacting the cell with variant Cas9 proteins or fusion proteins as described herein, and at least one guide RNA having a region complementary to a selected portion of the genome of the cell with optimal nucleotide spacing at the genomic target site. The methods can include contacting the cell with a nucleic acid encoding the Cas9 protein and the guide RNA, e.g., in a single vector; contacting the cell with a nucleic acid encoding the Cas9 protein and a nucleic acid encoding the guide RNA, e.g., in multiple vectors; and contacting the cell with a complex of purified Cas9 protein and synthetic or purified gRNA, inter alia. In some embodiments, the cell stably expresses one or both of the gRNA or the variant protein/fusion protein, and the other element is transfected or introduced into the cell. For example, the cell may stably express a variant protein or fusion protein as described herein, and the methods can include contacting the cell with a synthetic gRNA, a purified recombinantly produced gRNA, or a nucleic acid encoding the gRNA. In some embodiments, the variant protein or fusion protein comprises one or more of a nuclear localization sequence, cell penetrating peptide sequence, and/or affinity tag.

Also provided herein are methods for altering, e.g., selectively altering, an isolated dsDNA molecule in vitro by contacting the dsDNA with a purified variant protein or fusion protein as described herein, and a guide RNA having a region complementary to a selected portion of the dsDNA molecule.

Unless otherwise defined, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs. Methods and materials are described herein for use in the present invention; other, suitable methods and materials known in the art can also be used. The materials, methods, and examples are illustrative only and not intended to be limiting. All publications, patent applications, patents, sequences, database entries, and other references mentioned herein are incorporated by reference in their entirety. In case of conflict, the present specification, including definitions, will control.

Other features and advantages of the invention will be apparent from the following detailed description and figures, and from the claims.

DESCRIPTION OF DRAWINGS

FIGS. 1A-E|Identification and characterization of SpCas9 variants bearing mutations in residues that form non-specific DNA contacts. A, Schematic depicting wild-type SpCas9 recognition of the target DNA:sgRNA duplex, based on PDB 4OOG and 4UN3 (adapted from refs. 31 and 32, respectively). B, Characterization of SpCas9 variants that contain alanine substitutions in positions that form hydrogen bonds to the DNA backbone. Wild-type SpCas9 and variants were assessed using the human cell EGFP disruption assay when programmed with a perfectly matched sgRNA or four other sgRNAs that encode mismatches to the target site. Error bars represent s.e.m. for n=3; mean level of background EGFP loss represented by red dashed line (for this panel and panel C). C and D, On-target activities of wild-type SpCas9 and SpCas9-HF1 across 24 sites assessed by EGFP disruption assay (panel C) and 13 endogenous sites by T7E1. assay (panel D). Error bars represent s.e.m. for n=3. E, Ratio of on-target activity of SpCas9-HF1 to wild-type SpCas9 (from panels C and D).

FIG. 2A-C|Genome-wide specificities of wild-type SpCas9 and SpCas9-HF1 with sgRNAs for standard target sites. A, Off-target sites of wild-type SpCas9 and SpCas9-HF1 with eight sgRNAs targeted to endogenous human genes, as determined by GUIDE-seq. Read counts represent a measure of cleavage frequency at a given site; mismatched positions within the spacer or PAM are highlighted in color. B, Summary of the total number of genome-wide off-target sites identified by GUIDE-seq for wild-type SpCas9 and SpCas9-HF1 from the eight sgRNAs used in panel A. C, Off-target sites identified for wild-type SpCas9 and SpCas9-HF1 for the eight sgRNAs, binned according to the total number of mismatches (within the protospacer and PAM) relative to the on-target site.

FIG. 3A-C|Validation of SpCas9-HF1 specificity improvements by targeted deep sequencing of off-target sites identified by GUIDE-seq. A, Mean on-target percent modification determined by deep sequencing for wild-type SpCas9 and SpCas9-HF1 with six sgRNAs from FIG. 2. Error bars represent s.e.m. for n=3. B, Percentage of deep sequenced on-target sites and GUIDE-seq detected off-target sites that contain indel mutations. Triplicate experiments are plotted for wild-type SpCas9, SpCas9-HF1, and control conditions. Filled circles below the x-axis represent replicates for which no insertion or deletion mutations were observed, Off-target sites that could not be amplified by PCR are shown in red text with an asterisk. Hypothesis testing using a one-sided Fisher exact test with pooled read counts found significant differences (p<0.05 after adjusting for multiple comparisons using the Benjamini-Hochberg method) for comparisons between SpCas9-HF1 and the control condition only at EMX1-1 off-target 1 and FANCF-3 off-target 1. Significant differences were also found between wild-type SpCas9 and SpCas9-HF1 at all off-target sites, and between wild-type SpCas9 and the control condition at all off-target sites except RUNX1-1 off-target 2. C, Scatter plot of the correlation between GUIDE-seq read counts (from FIG. 2A) and mean percent modification determined by deep sequencing at on- and off-target cleavage sites with wild-type SpCas9.

FIG. 4A-C|Genome-wide specificities of wild-type SpCas9 and SpCas9-HF1 with sgRNAs for non-standard, repetitive sites. A, GUIDE-seq specificity profiles of wild-type SpCas9 and SpCas9-HF1 using two sgRNAs known to cleave large numbers of off-target sites (Fu et al., Nat Biotechnol 31, 822-826 (2013); Tsai et al., Nat Biotechnol 33, 187-197 (2015)). GUIDE-seq read counts represent a measure of cleavage efficiency at a given site; mismatched positions within the spacer or PAM are highlighted in color; red circles indicate sites likely to have the indicated bulge (Lin et al., Nucleic Acids Res 42, 7473-7485 (2014)) at the sgRNA-DNA interface; blue circles indicate sites that may have an alternative gapped alignment relative to the one shown (see FIG. 8). B, Summary of the total number of genome-wide off-target sites identified by GUIDE-seq for wild-type SpCas9 and SpCas9-HF1 from the two sgRNAs used in panel A. C, Off-target sites identified with wild-type SpCas9 or SpCas9-HF1 for VEGFA sites 2 and 3, binned according to the total number of mismatches (within the protospacer and PAM) relative to the on-target site. Off-target sites marked with red circles in panel A are not included in these counts; sites marked with blue circles in panel A are counted with the number of mismatches in the non-gapped alignment.

FIG. 5A-D|Activities of SpCas9-HF1 derivatives bearing additional substitutions. A, Human cell EGFP disruption activities of wild-type SpCas9, SpCas9-HF1, and SpCas9-HF1-derivative variants with eight sgRNAs. SpCas9-HF1 harbors N497A, R661A, Q695, and Q926A mutations; HF2=HF1+D1135E; HF3=HF1+L169A; HF4=HF1+Y450A. Error bars represent s.e.m. for n=3; mean level of background EGFP loss represented by the red dashed line. B, Summary of the on-target activity when using SpCas9-HF variants compared to wild-type SpCas9 with the eight sgRNAs from panel a. The median and interquartile range are shown; the interval showing >70% of wild-type activity is highlighted in green. C, Mean percent modification by SpCas9 and HF variants at the FANCF site 2 and VEGFA site 3 on-target sites, as well as off-target sites from FIGS. 2A and 4A resistant to the effects of SpCas9-HF1. Percent modification determined by T7E1 assay; background indel percentages were subtracted for all experiments. Error bars represent s.e.m. for n=3. D, Specificity ratios of wild-type SpCas9 and HF variants with the FANCF site 2 or VEGFA site 3 sgRNAs, plotted as the ratio of on-target to off-target activity (from panel C).

FIGS. 5E-F|Genome-wide specificities of SpCas9-HF1, -HF2, and -HF4 with sgRNAs that have off-target sites resistant to the effects of SpCas9-HF1. E, Mean GUIDE-seq tag integration at the intended on-target site for GUIDE-seq experiments in panel F. SpCas9-HF1=N497A/R661A/Q695A/Q926A; HF2=HF1+D1135E; HF4=HF1+Y450A. Error bars represent s.e.m. for n=3. F, GUIDE-seq identified off-target sites of SpCas9-HF1, -HF2, or -HF4 with either the FANCF site 2 or VEGFA site 3 sgRNAs. Read counts represent a measure of cleavage frequency at a given site; mismatched positions within the spacer or PAM are highlighted in color. The fold-improvement in off-target discrimination was calculated by normalizing the off-target read counts for an SpCas9-HF variant to the read counts at the on-target site prior to comparison between SpCas9-HF variants.

FIG. 6A-B SpCas9 interaction with the sgRNA and target DNA. A, Schematic illustrating the SpCas9:sgRNA complex, with base pairing between the sgRNA and target DNA. B, Structural representation of the SpCas9:sgRNA complex bound to the target DNA, from PDB: 4UN3 (ref. 32). The four residues that form hydrogen bond contacts to the target-strand DNA backbone are highlighted in blue; the HNH domain is hidden for visualization purposes.

FIG. 7A-D|On-target activity comparisons of wild-type and SpCas9-HF1 with various sgRNAs used for GUIDE-seq experiments. A and C, Mean GUIDE-seq tag integration at the intended on-target site for GUIDE-seq experiments shown in FIGS. 2A and 4A (panels 7A and 7C, respectively), quantified by restriction fragment length polymorphism assay. Error bars represent s.e.m. for n=3. b and d, Mean percent modification at the intended on-target site for GUIDE-seq experiments shown in FIGS. 2A and 4A (panels 7B and 7D, respectively), detected by T7E1 assay. Error bars represent s.e.m. for n=3.

FIG. 8|Potential alternate alignments for VEGFA site 2 off-target sites. Ten VEGFA site 2 off-target sites identified by GUIDE-seq (left) that may potentially be recognized as off-target sites that contain single nucleotide gaps (Lin et al., Nucleic Acids Res 42, 7473-7485 (2014))) (right), aligned using Geneious (Kearse et al., Bioinformatics 28, 1647-1649 (2012)) version 8.1.6.

FIG. 9|Activities of wild-type SpCas9 and SpCas9-HF1 with truncated sgRNAs14. EGFP disruption activities of wild-type SpCas9 and SpCas9-HF1 using full-length or truncated sgRNAs targeted to four sites in EGFP. Error bars represent s.e.m. for n=3; mean level of background EGFP loss in control experiments is represented by the red dashed line

FIG. 10|Wild-type SpCas9 and SpCas9-HF1 activities with sgRNAs bearing 5′-mismatched guanine bases. EGFP disruption activities of wild-type SpCas9 and SpCas9-HF1 with sgRNAs targeted to four different sites. For each target site, sgRNAs either contain the matched non-guanine 5′-base or a 5′-guanine that is intentionally mismatched.

FIG. 11|Titrating the amount of wild-type SpCas9 and SpCas9-HF1 expression plasmids. Human cell EGFP disruption activities from transfections with varying amounts of wild-type and SpCas9-HF1 expression plasmids. For all transfections, the amount of sgRNA-containing plasmid was fixed at 250 ng. Two sgRNAs targeting separate sites were used; Error bars represent s.e.m. for n=3; mean level of background EGFP loss in negative controls is represented by the red dashed line.

FIG. 12A-D|Altering the PAM recognition specificity of SpCas9-HF1. A, Comparison of the mean percent modification of on-target endogenous human sites by SpCas9-VQR (ref. 15) and an improved SpCas9-VRQR using 8 sgRNAs, quantified by T7E1 assay. Both variants are engineered to recognize an NGAN PAM. Error bars represent s.e.m. for n=2 or 3. B, On-target EGFP disruption activities of SpCas9-VQR and SpCas9-VRQR compared to their -HF1 counterparts using eight sgRNAs. Error bars represent s.e.m. for n=3; mean level of background EGFP loss in negative controls represented by the red dashed line. C, Comparison of the mean on-target percent modification by SpCas9-VQR and SpCas9-VRQR compared to their -HF1 variants at eight endogenous human gene sites, quantified by T7E1 assay. Error bars represent s.e.m. for n=3; ND, not detectable. D, Summary of the fold-change in on-target activity when using SpCas9-VQR or SpCas9-VRQR compared to their corresponding -HF1 variants (from panels B and C). The median and interquartile range are shown; the interval showing >70% of wild-type activity is highlighted in green.

FIGS. 13A-B|Activities of wild-type SpCas9, SpCas9-HF1, and wild-type SpCas9 derivatives bearing one or more alanine substitutions at positions that can potentially contact the non-target DNA strand. A and B, Nucleases were assessed using the EGFP disruption assay, with an sgRNA that is perfectly matched to a site in the EGFP gene as well as an sgRNA that is intentionally mismatched at positions 11 and 12 (panel A) or positions 9 and 10 (panel B). Mismatched positions are numbered with position 20 being the most PAM-distal position; the red dashed line represents background levels of EGFP disruption; HF1=SpCas9 with N497A/R661A/Q695A/Q926A substitutions.

FIGS. 14A-B|Activity of wild-type SpCas9, SpCas9-HF1, and SpCas9-HF1 derivatives bearing one or more alanine substitutions at positions that can potentially contact the non-target DNA strand. A and B, Nucleases were assessed using the EGFP disruption assay, with an sgRNA that is perfectly matched to a site in the EGFP gene as well as an sgRNA that is intentionally mismatched at positions 11 and 12 (panel A) or positions 9 and 10 (panel B). Mismatched positions are numbered with position 20 being the most PAM-distal position; the red dashed line represents background levels of EGFP disruption; HF1=SpCas9 with N497A/R661A/Q695A/Q926A substitutions.

FIG. 15|Activity of wild-type SpCas9, SpCas9-HF1, and SpCas9(Q695A/Q926A) derivatives bearing one or more alanine substitutions at positions that can potentially contact the non-target DNA strand. Nucleases were assessed using the EGFP disruption assay, with an sgRNA that is perfectly matched to a site in the EGFP gene as well as an sgRNA that is intentionally mismatched at positions 11 and 12. Mismatched positions are numbered with position 20 being the most PAM-distal position; the red dashed line represents background levels of EGFP disruption; HF1=SpCas9 with N497A/R661A/Q695A/Q926A substitutions; Dbl=SpCas9 with Q695A/Q926A substitutions.

FIG. 16|Activities of wild-type SpCas9, SpCas9-HFF1, and eSpCas9-1.1 using a matched sgRNA and sgRNAs with single mismatches at each position in the spacer. Nucleases were assessed using the EGFP disruption assay, with an sgRNA that is perfectly matched to a site in the EGFP gene (“matched”) as well as sgRNAs that are intentionally mismatched at the positions indicated. Mismatched positions are numbered with position 20 being the most PAM-distal position. SpCas9-HF1=N497A/R661A/Q695A/Q926A, and eSP1.1=K848A/K1003A/R1060A.

FIGS. 17A-B|Activities of wild-type SpCas9 and variants using a matched sgRNA and sgRNAs with single mismatches at various positions in the spacer. (A) The activities of SpCas9 nucleases containing combinations of alanine substitutions (directed to positions that may potentially contact the target or non-target DNA strands) were assessed using the EGFP disruption assay, with an sgRNA that is perfectly matched to a site in the EGFP gene (“matched”) as well as sgRNAs that are intentionally mismatched at the indicated spacer positions. (B) A subset of these nucleases from (a) were tested using the remainder of all possible singly mismatched sgRNAs for the matched on-target site. Mismatched positions are numbered with position 20 being the most PAM-distal position. min=mismatch, WT=wild-type, Db=Q695A/Q926A, HF1=N497A/R661A/Q695A/Q926A, 1.0=K810A/K1003A/R1060A, and 1.1=K848A/K1003A/R1060A.

FIG. 18|Activities of wild-type SpCas9 and variants using a matched sgRNA and sgRNAs with mismatches at various individual positions in the spacer. The activities of SpCas9 nucleases containing combinations of alanine substitutions (directed to positions that may potentially contact the target or non-target DNA strands), were assessed using the EGFP disruption assay with an sgRNA that is perfectly matched to a site in the EGFP gene (“matched”) as well as sgRNAs that are intentionally mismatched at the indicated positions. Db=Q695A/Q926A, HF1=N497A/R661A/Q695A/Q926A.

FIGS. 19A-B|Activities of wild-type SpCas9 and variants using a matched sgRNA and sgRNAs with mismatches at various individual positions in the spacer. (A) The on-target activities of SpCas9 nucleases containing combinations of alanine substitutions (directed to positions that may potentially contact the target or non-target DNA strands), were assessed using the EGFP disruption assay with two sgRNAs that are perfectly matched to a site in the EGFP gene. (B) A subset of these nucleases from (a) were tested with sgRNAs containing mismatches at positions 12, 14, 16, or 18 (of sgRNA ‘site 1’) in their spacer sequence to determine whether intolerance to mismatches was imparted by these substitutions. Db=Q695A/Q926A, HF1=N497A/R661A/Q695A/Q926A.

FIG. 20|Structural comparison of SpCas9 (top) and SaCas9 (bottom) illustrating the similarity between the positions of the mutations in the quadruple mutant constructs (shown in yellow sphere representation). Also, shown in pink sphere representation are other residues that contact the DNA backbone.

FIGS. 21A-B|Activity of wild-type SaCas9 and SaCas9 derivatives bearing one or more alanine substitutions. A and B, SaCas9 substitutions were directed to positions that may potentially contact the target DNA strand (panel A) or have previously been shown to influence PAM specificity (panel B). Nucleases were assessed using the EGFP disruption assay, with an sgRNA that is perfectly matched to a site in the EGFP gene as well as an sgRNA that is intentionally mismatched at positions 11 and 12. Mismatched positions are numbered with position 20 being the most PAM-distal position; the red dashed line represents background levels of EGFP disruption.

FIGS. 22A-B|Activities of wild-type (WT) SaCas9 and SaCas9 derivatives bearing one or more alanine substitutions at residues that may potentially contact the target DNA strand. A and B, Nucleases were assessed using the EGFP disruption assay, with an sgRNA that is perfectly matched to a site in the EGFP gene (“matched”) and with an sgRNA that is intentionally mismatched at positions 19 and 20. Mismatched positions are numbered with position 20 being the most PAM-distal position.

FIG. 23|Activities of wild-type(WT) SaCas9 and SaCas9 variants bearing triple combinations of alanine substitutions at residues that may potentially contact the target DNA strand. Nucleases were assessed using the EGFP disruption assay. Four different sgRNAs were used (matched #1-4), with each of the four target sites also being tested with mismatched sgRNAs known to be efficiently used by wild-type SaCas9. Mismatched sgRNAs for each site are shown to the right of each matched sgRNA (for example, the only mismatched sgRNA for matched site 3 is mm 11 & 12). Mismatched positions are numbered with position 21 being the most PAM-distal position; mm, mismatch.

FIGS. 24A-B|Activities of wild-type (WT) SaCas9 and SaCas9 derivatives bearing one or more alanine substitutions at residues that may potentially contact the target DNA strand. A and B, SaCas9 variants bearing double (A) or triple (B) combinations substitutions were assessed against matched and singly mismatched endogenous human gene target sites using the T7E1 assay. Matched ‘on-target’ sites are named according to their gene target site sgRNA number from Kleinstiver et al., Nature Biotechnology 2015. Mismatched sgRNAs are numbered with the mismatch occurring at position 21, the most PAM-distal position; mismatched sgRNAs are derived from the matched on-target site that is listed to the left of the mismatched sgRNA.

DETAILED DESCRIPTION

A limitation of the CRISPR-Cas9 nucleases is their potential to induce undesired “off-target” mutations at imperfectly matched target sites (see, for example, Tsai et al., Nat Biotechnol. 2015), in some cases with frequencies rivaling those observed at the intended on-target site (Fu et al., Nat Biotechnol. 2013). Previous work with CRISPR-Cas9 nucleases has suggested that reducing the number of sequence-specific interactions between the guide RNA (gRNA) and the spacer region of a target site can reduce mutagenic effects at off-target sites of cleavage in human cells (Fu et al., Nat Biotechnol. 2014).

This was earlier accomplished by truncating gRNAs at their 5′ ends by 2 or 3 nts and it was hypothesized that the mechanism of this increased specificity was a decrease in the interaction energy of the gRNA/Cas9 complex so that it was poised with just enough energy to cleave the on-target site, making it less likely to have enough energy to cleave off-target sites where there would presumably be an energetic penalty due to mismatches in the target DNA site (WO2015/099850).

It was hypothesized that off-target effects (at DNA sites that are imperfect matches or mismatches with the intended target site for the guide RNA) of SpCas9 might be minimized by decreasing non-specific interactions with its target DNA site. SpCas9-sgRNA complexes cleave target sites composed of an NGG PAM sequence (recognized by SpCas9) (Deltcheva, E. et al. Nature 471, 602-607 (2011); Jinek, M. et al. Science 337, 816-821 (2012); Jiang, W., et al., Nat Biotechnol 31, 233-239 (2013); Sternberg, S. H., et al., Nature 507, 62-67 (2014)) and an adjacent 20 bp protospacer sequence (which is complementary to the 5′ end of the sgRNA) (Jinek, M. et al. Science 337, 816-821(2012); Jinek, M. et al. Elife 2, e00471 (2013); Mali, P. et al., Science 339, 823-826(2013); Cong, L. et al., Science 339, 819-823 (2013)). It was previously theorized that the SpCas9-sgRNA complex may possess more energy than is needed for recognizing its intended target DNA site, thereby enabling cleavage of mismatched off-target sites (Fu, Y., et al., Nat Biotechnol 32, 279-284 (2014)). One can envision that this property might be advantageous for the intended role of Cas9 in adaptive bacterial immunity, giving it the capability to cleave foreign sequences that may become mutated. This excess energy model is also supported by previous studies demonstrating that off-target effects can be reduced (but not eliminated) by decreasing SpCas9 concentration (Hsu, P.D. et al. Nat Biotechnol 31, 827-832 (2013); Pattanayak, V. et al. Nat Biotechnol 31, 839-843 (2013)) or by reducing the complementarity length of the sgRNA (Fu, Y., et al., Nat Biotechnol 32, 279-284 (2014), although other interpretations for this effect have also been proposed (Josephs, E. A. et al. Nucleic Acids Res 43, 8924-8941 (2015); Sternberg, S. H., et al. Nature 527, 110-113 (2015); Kiani, S. et al. Nat Methods 12, 1051-1054 (2015))). Structural data suggests that the SpCas9-sgRNA-target DNA complex may be stabilized by several SpCas9-mediated DNA contacts, including direct hydrogen bonds made by four SpCas9 residues (N497, R661, Q695, Q926) to the phosphate backbone of the target DNA strand (Nishimasu, H. et al. Cell 156, 935-949 (2014); Anders, C., et al. Nature 513, 569-573 (2014)) (FIG. 1a and FIGS. 6a and 6b ). The present inventors envisioned that disruption of one or more of these contacts might energetically poise the SpCas9-sgRNA complex at a level just sufficient to retain robust on-target activity but with a diminished ability to cleave mismatched off-target sites.

As described herein, Cas9 proteins can be engineered to show increased specificity, theoretically by reducing the binding affinity of Cas9 for DNA. Several variants of the widely used Streptococcus pyogenes Cas9 (SpCas9)were engineered by introducing individual alanine substitutions into various residues in SpCas9 that might be expected to interact with phosphates on the DNA backbone using structural information, bacterial selection-based directed evolution, and combinatorial design. The variants were further tested for cellular activity using a robust E. coli-based screening assay to assess the cellular activities of these variants; in this bacterial system, cell survival depended on cleavage and subsequent destruction of a selection plasmid containing a gene for the toxic gyrase poison ccdB and a 23 base pair sequence targeted by a gRNA and SpCas9, and led to identification of residues that were associated with retained or lost activity. In addition, another SpCas9 variant was identified and characterized, which exhibited improved target specificity in human cells.

Furthmore, activities of single alanine substitution mutants of SpCas9 as assessed in the bacterial cell-based system indicated that survival percentages between 50-100% usually indicated robust cleavage, whereas 0% survival indicated that the enzyme had been functionally compromised. Additional mutations of SpCas9 were then assayed in bacteria to include: R63A, R66A, R69A, R70A, R71A, Y72A, R74A, R75A, K76A, N77A, R78A, R115A, H160A, K163A, R165A, L169A, R403A, T404A, F405A, N407A, R447A, N497A, I448A, Y450A, S460A, M495A, K510A, Y515A, R661A, M694A, Q695A, H698A, Y1013A, V1015A, R1122A, K1123A, K1124A, K1158A, K1185A, K1200A, S1216A, Q1221A, K1289A, R1298A, K1300A, K1325A, R1333A, K1334A, R1335A, and T1337A. With the exception of 2 mutants (R69A and F405A) that had <5% survival in bacteria, all of these additional single mutations appeared to have little effect on the on-target activity of SpCas9 (>70% survival in the bacterial screen).

To further determine whether the variants of Cas9 identified in the bacterial screen functioned efficiently in human cells, various alanine substitution Cas9 mutants were tested using a human U2OS cell-based EGFP-disruption assay. In this assay, successful cleavage of a target site in the coding sequence of a single integrated, constitutively expressed EGFP gene led to the induction of indel mutations and disruption of EGFP activity, which was quantitatively assessed by flow cytometry (see, for example, Reyon et al., Nat Biotechnol. 2012 May; 30(5):460-5).

These experiments show that the results obtained in the bacterial cell-based assay correlate well with nuclease activities in human cells, suggesting that these engineering strategies could be extended to Cas9s from other species and different cells. Thus these findings provide support for SpCas9 and SaCas9 variants, referred to collectively herein as “variants” or “the variants”.

All of the variants described herein can be rapidly incorporated into existing and widely used vectors, e.g., by simple site-directed mutagenesis, and because they require only a small number of mutations, the variants should also work with other previously described improvements to the SpCas9 platform (e.g., truncated sgRNAs (Tsai et al., Nat Biotechnol 33, 187-197 (2015); Fu et al., Nat Biotechnol 32, 279-284 (2014)), nickase mutations (Mali et al., Nat Biotechnol 31, 833-838 (2013); Ran et al., Cell 154, 1380-1389(2013)), FokI-dCas9 fusions (Guilinger et al., Nat Biotechnol 32, 577-582 (2014); Tsai et al., Nat Biotechnol 32, 569-576 (2014); WO2014144288); and engineered CRISPR-Cas9 nucleases with altered PAM specificities (Kleinstiver et al., Nature. 2015 Jul. 23; 523(7561):481-5).

Thus, provided herein are Cas9 variants, including SpCas9 variants. The SpCas9 wild type sequence is as follows:

(SEQ ID NO: 1)         10         20         30         40 MDKKYSIGLD IGINSVGWAV ITDEYKVPSK KFKVLGNTDR         50         60         70         80 HSIKKNLIGA LLFDSGETAE ATRLKRTARR RYTRRKNRIC         90        100        110        120 YLQEIFSNEM AKVDDSFFHR LEESFLVEED KKHERHPIFG        130        140        150        160 NIVDEVAYHE KYPTIYHLRK KLVDSTDKAD LRLIYLALAH        170        180        190        200 MIKFRGHFLI EGDLNPDNSD VDKLFIQLVQ TYNQLFEENP        210        220        230        240 INASGVDAKA ILSARLSKSR RLENLIAQLP GEKKNGLFGN        250        260        270        280 LIALSLGLTP NFKSNFDLAE DAKLQLSKDT YDDDLDNLLA        290        300        310        320 QIGDQYADLF LAAKNLSDAI LLSDILRVNT EITKAPLSAS        330        340        350        360 MIKRYDEHHQ DLTLLKALVR QQLPEKYKEI FFDQSKNGYA        370        380        390        400 GYIDGGASQE EFYKFIKPIL EKMDGTEELL VKLNREDLLR        410        420        430        440 KQRTFDNGSI PHQIHLGELH AILRRQEDFY PFLKDNREKI        450        460        470        480 EKILTFRIPY YVGPLARGNS RFAWMTRKSE ETITPWNFEE        490        500        510        520 VVDKGASAQS FIERMTNFDK NLPNEKVLPK HSLLYEYFTV        530        540        550        560 YNELTKVKYV TEGMRKPAFL SGEQKKAIVD LLFKTNRKVT        570        580        590        600 VKQLKEDYFK KIECFDSVEI SGVEDRFNAS LGTYHDLLKI        610        620        630        640 IKDKDFLDNE ENEDILEDIV LTLTLFEDRE MIEERLKTYA        650        660        670        680 HLFDDKVMKQ LKRRRYTGWG RLSRKLINGI RDKQSGKTIL        690        700        710        720 DFLKSDGFAN RNFMQLIHDD SLTFKEDIQK AQVSGQGDSL        730        740        750        750 HEHIANLAGS PAIKKGILQT VKVVDELVKV MGRHKPENIV        770        780        790        800 IEMARENQTT QKGQKNSRER MKRIEEGIKE LGSQILKEHP        810        820        830        840 VENTQLQNEK LYLYYLQNGR DMYVDQELDI NRLSDYDVDH        850        860        870        880 IVPQSFLKDD SIDNKVLTRS DKNRGKSDNV PSEEVVKKMK        890        900        910        920 NYWRQLLNAK LITQRKFDNL TKAERGGLSE LDKAGFIKRQ        930        940        950        960 LVETRQITKH VAQILDSRMN TKYDENDKLI REVKVITLKS        970        980        990       1000 KLVSDFRKDF QFYKVREINN YHHAHDAYLN AVVGTALIKK       1010       1020       1030       1040 YPKLESEFVY GDYKVYDVRK MIAKSEQEIG KATAKYFFYS       1050       1060       1070       1080 NIMNFFKTEI TLANGEIRKR PLIETNGETG EIVWDKGRDF       1090       1100       1110       1120 ATVRKVLSMP QVNIVKKTEV QTGGFSKESI LPKRNSDKLI       1130       1140       1150       1160 ARKKDWDPKK YGGFDSPTVA YSVLVVAKVE KGKSKKLKSV       1170       1180       1190       1200 KELLGITIME RSSFEKNPID FLEAKGYKEV KKDLIIKLPK       1210       1220       1230       1240 YSLFELENGR KRMLASAGEL QKGNELALPS KYVNFLYLAS       1250       1260       1270       1280 HYEKLKGSPE DNEQKQLFVE QHKHYLDEII EQISEFSKRV       1290       1300       1310       1320 ILADANLDKV LSAYNKHRDK PIREQAENII HLFTLTNLGA       1330       1340       1350       1360 PAAFKYFDTT IDRKRYTSTK EVLDATLIHQ SITGLYETRI DLSQLGGD

The SpCas9 variants described herein can include the amino acid sequence of SEQ ID NO:1, with mutations (i.e., replacement of the native amino acid with a different amino acid, e.g., alanine, glycine, or serine), at one or more of the following positions: N497, R661, Q695, Q926 (or at positions analogous thereto). In some embodiments, the SpCas9 variants are at least 80%, e.g., at least 85%, 90%, or 95% identical to the amino acid sequence of SEQ ID NO:1, e.g., have differences at up to 5%, 10%, 15%, or 20% of the residues of SEQ ID NO:1 replaced, e.g., with conservative mutations, in addition to the mutations described herein. In preferred embodiments, the variant retains desired activity of the parent, e.g.,the nuclease activity (except where the parent is a nickase or a dead Cas9), and/or the ability to interact with a guide RNA and target DNA).

To determine the percent identity of two nucleic acid sequences, the sequences are aligned for optimal comparison purposes (e.g., gaps can be introduced in one or both of a first and a second amino acid or nucleic acid sequence for optimal alignment and non-homologous sequences can be disregarded for comparison purposes). The length of a reference sequence aligned for comparison purposes is at least 80% of the length of the reference sequence, and in some embodiments is at least 90% or 100%. The nucleotides at corresponding amino acid positions or nucleotide positions are then compared. When a position in the first sequence is occupied by the same nucleotide as the corresponding position in the second sequence, then the molecules are identical at that position (as used herein nucleic acid “identity” is equivalent to nucleic acid “homology”). The percent identity between the two sequences is a function of the number of identical positions shared by the sequences, taking into account the number of gaps, and the length of each gap, which need to be introduced for optimal alignment of the two sequences. Percent identity between two polypeptides or nucleic acid sequences is determined in various ways that are within the skill in the art, for instance, using publicly available computer software such as Smith Waterman Alignment (Smith, T. F. and M. S. Waterman (1981) J Mol Biol 147:195-7); “BestFit” (Smith and Waterman, Advances in Applied Mathematics, 482-489 (1981)) as incorporated into GeneMatcher Plus™, Schwarz and Dayhof (1979) Atlas of Protein Sequence and Structure, Dayhof, M. O., Ed, pp 353-358; BLAST program (Basic Local Alignment Search Tool; (Altschul, S. F., W. Gish, et al. (1990) J Mol Biol 215:403-10), BLAST-2, BLAST-P, BLAST-N, BLAST-X, WU-BLAST-2, ALIGN, ALIGN-2, CLUSTAL, or Megalign (DNASTAR) software. In addition, those skilled in the art can determine appropriate parameters for measuring alignment, including any algorithms needed to achieve maximal alignment over the length of the sequences being compared. In general, for proteins or nucleic acids, the length of comparison can be any length, up to and including full length (e.g., 5%, 10%, 20%, 30%, 40%, 50%, 60%, 70%, 80%, 90%, 95%, or 100%). For purposes of the present compositions and methods, at least 80% of the full length of the sequence is aligned.

For purposes of the present invention, the comparison of sequences and determination of percent identity between two sequences can be accomplished using a Blossum 62 scoring matrix with a gap penalty of 12, a gap extend penalty of 4, and a frameshift gap penalty of 5.

Conservative substitutions typically include substitutions within the following groups: glycine, alanine; valine, isoleucine, leucine; aspartic acid, glutamic acid, asparagine, glutamine; serine, threonine; lysine, arginine; and phenylalanine, tyrosine.

In some embodiments, the SpCas9 variants include one of the following sets of mutations: N497A/R661A/Q695/Q926A (quadruple alanine mutant); Q695A/Q926A (double alanine mutant); R661A/Q695A/Q926A and N497A/Q695A/Q926A (triple alanine mutants). In some embodiments, the additional substitution mutations at L169 and/or Y450 might be added to these double-, triple, and quadruple mutants or added to single mutants bearing substitutions at Q695 or Q926. In some embodiments, the mutants have alanine in place of the wild type amino acid. In some embodiments, the mutants have any amino acid other than arginine or lysine (or the native amino acid).

In some embodiments, the SpCas9 variants also include one of the following mutations, which reduce or destroy the nuclease activity of the Cas9: D10, E762, D839, H983, or D986 and H840 or N863, e.g., D10A/D10N and H840A/H840N/H840Y, to render the nuclease portion of the protein catalytically inactive; substitutions at these positions could be alanine (as they are in Nishimasu al., Cell 156, 935-949 (2014)), or other residues, e.g., glutamine, asparagine, tyrosine, serine, or aspartate, e.g., E762Q, H983N, H983Y, D986N, N863D, N863S, or N863H (see WO 2014/152432). In some embodiments, the variant includes mutations at D10A or H840A (which creates a single-strand nickase), or mutations at D10A and H840A (which abrogates nuclease activity; this mutant is known as dead Cas9 or dCas9).

The SpCas9 N497A/R661A/Q695A/R926A mutations have analogous residues in Staphylococcus aureus Cas9 (SaCas9); see FIG. 20. Mutations to the residues contacting the DNA or RNA backbone are expected to increase the specificity of SaCas9 as we've observed for SpCas9. Thus, also provided herein are SaCas9 variants.

The SaCas9 wild type sequence is as follows:

(SE0 ID NO: 2)         10         20         30         40 MKRNYILGLD IGITSVGYGI IDYETRDVID AGVRLFKEAN         50         60         70         80 VENNEGRRSK RGARRLKRRR RHRIQRVKKL LFDYNLLTDH         90        100        110        120 SELSGINPYE ARVKGLSQKL SEEEFSAALL HLAKRRGVHN        130        140        150        160 VNEVEEDTGN ELSTKEQISR NSKALEEKYV AELQLERLKK        170        180        190        200 DGEVRGSINR FKTSDYVKEA KQLLKVQKAY HQLDQSFIDT        210        220        230        240 YIDLLETRRT YYEGPGEGSP FGWKDIKEWY EMLMGHCTYF        250        260        270        280 PEELRSVKYA YNADLYNALN DLNNLVITRD ENEKLEYYEK        290        300        310        320 FQIIENVFKQ KKKPTLKQIA KEILVNEEDI KGYRVTSTGK        330        340        350        360 PEFTNLKVYH DIKDITARKE IIENAELLDQ IAKILTIYQS        370        380        390        400 SEDIQEELTN LNSELTQEEI EQISNLKGYT GTHNLSLKAI        410        420        420        440 NLILDELWHT NDNQIAIFNR LKLVPKKVDL SQQKEIPTTL        450        460        470        480 VDDFILSPVV KRSFIQSIKV INAIIKKYGL PNDIIIELAR        490        500        510        520 EKNSKDAQKM INEMQKRNRQ TNERIEEIIR TTGKENAKYL        530        540        550        560 IEKIKLHDMQ EGKCLYSLEA IPLEDLLNNP FNYEVDHIIP        570        580        590        600 RSVSFDNSFN NKVLVKQEEN SKKGNRTPFQ YLSSSDSKIS        610        620        630        640 YETFKKHILN LAKGKGRISK TKKEYLLEER DINRFSVQKD        650        660        670        680 FINRNLVDTR YATRGLMNLL RSYFRVNNLD VKVKSINGGF        690        700        710        720 TSFLRRKWKF KKERNKGYKH HAEDALIIAN ADFIFKEWKK        730        740        750        760 LDKAKKVMEN QMFEEKQAES MPEIETEQEY KEIFITPHQI        770        780        790        800 KHIKDFKDYK YSHRVDKKPN RELINDTLYS TRKDDKGNTL        810        820        830        840 IVNNLNGLYD KDNDKLKKLI NKSPEKLLMY HHDPQTYQKL        850        860        870        880 KLIMEQYGDE KNPLYKYYEE TGNYLTKYSK KDNGPVIKKI        890        900        910        920 KYYGNKLNAH LDITDDYPNS RNKVVKLSLK PYRFDVYLDN        930        940        950        960 GVYKFVTVKN LDVIKKENYY EVNSKCYEEA KKLKKISNQA        970        980        990       1000 EFIASFYNND LIKINGELYR VIGVNNDLLN RIEVNMIDIT       1010       1020       1030       1040 YREYLENMND KRPPRIIKTI ASKTQSIKKY STDILGNLYE       1050 VKSKKHPQII KKG

SaCas9 variants described herein include the amino acid sequence of SEQ ID NO:2, with mutations at one, two, three, four, five, or all six of the following positions: Y211, W229, R245, T392, N419, and/or R654, e.g., comprising a sequence that is at least 80% identical to the amino acid sequence of SEQ ID NO:2 with mutations at one, two, three, four five or six of the following positions: Y211, W229, R245, T392, N419, and/or R654.

In some embodiments, the variant SaCas9 proteins also comprise one or more of the following mutations: Y211A; W229A; Y230A; R245A; T392A; N419A; L446A; Y651A; R654A; D786A; T787A; Y789A; T882A; K886A; N888A; A889A; L909A; N985A; N986A; R991A; R1015A; N44A; R45A; R51A; R55A; R59A; R60A; R116A; R165A; N169A; R208A; R209A; Y211A; T238A; Y239A; K248A; Y256A; R314A; N394A; Q414A; K57A; R61A; H111A; K114A; V164A; R165A; L788A; S790A; R792A; N804A; Y868A; K870A; K878A; K879A; K881A; Y897A; R901A; K906A.

In some embodiments, variant SaCas9 proteins comprise one or more of the following additional mutations: Y211A, W229A, Y230A, R245A, T392A, N419A, L446A, Y651A, R654A, D786A, T787A, Y789A, T882A, K886A, N888A, A889A, L909A, N985A, N986A, R991A, R1015A, N44A, R45A, R51A, R55A, R59A, R60A, R116A, R165A, N169A, R208A, R209A, Y211A , T238A, Y239A, K248A, Y256A, R314A, N394A, Q414A, K57A, R61A, H111A, K114A, V164A, R165A, L788A, S790A, R792A, N804A, Y868A, K870A, K878A, K879A, K881A, Y897A, R901A, K906A.

In some embodiments, the variant SaCas9 proteins comprise multiple substitution mutations: R245/T392/N419/R654 and Y221/R245/N419/R654 (quadruple variant mutants); N419/R654, R245/R654, Y221/R654, and Y221/N419 (double mutants); R245/N419/R654, Y211/N419/R654, and T392/N419/R654 (triple mutants). In some embodiments the mutants contain alanine in place of the wild type amino acid.

In some embodiments, the variant SaCas9 proteins also comprise mutations at E782K, K929R, N968K, and/or R1015H. For example, the KKH variant (E782K/N968K/R1015H), the KRH variant (E782K/K929R/R1015H), or the KRKH variant (E782K/K929R/N968K/R1015H)]

In some embodiments, the variant SaCas9 proteins also comprise one or more mutations that decrease nuclease activity selected from the group consisting of mutations at D10, E477, D556, H701; or D704; and at H557 or N580.

In some embodiments, the mutations are: (i) D10A or D10N, (ii) H557A, H557N, or H557Y, (iii) N580A, and/or (iv) D556A.

Also provided herein are isolated nucleic acids encoding the Cas9 variants, vectors comprising the isolated nucleic acids, optionally operably linked to one or more regulatory domains for expressing the variant proteins, and host cells, e.g., mammalian host cells, comprising the nucleic acids, and optionally expressing the variant proteins.

The variants described herein can be used for altering the genome of a cell; the methods generally include expressing the variant proteins in the cells, along with a guide RNA having a region complementary to a selected portion of the genome of the cell. Methods for selectively altering the genome of a cell are known in the art, see, e.g., U.S. Pat. No. 8,993,233; US 20140186958; U.S. Pat. No. 9,023,649; WO/2014/099744; WO 2014/089290; WO2014/144592; WO144288; WO2014/204578; WO2014/152432; WO2115/099850; U.S. Pat. No. 8,697,359; US20160024529; US20160024524; US20160024523; US20160024510; US20160017366; US20160017301; US20150376652; US20150356239; US20150315576; US20150291965; US20150252358; US20150247150; US20150232883; US20150232882; US20150203872; US20150191744; US20150184139; US20150176064; US20150167000; US20150166969; US20150159175; US20150159174; US20150093473; US20150079681; US20150067922; US20150056629; US20150044772; US20150024500; US20150024499; US20150020223; US20140356867; US20140295557; US20140273235; US20140273226; US20140273037; US20140189896; US20140113376; US20140093941; US20130330778; US20130288251; US20120088676; US20110300538; US20110236530; US20110217739, US20110002889; US20100076057; US20110189776; US20110223638; US20130130248; US20150050699; US20150071899; US20150050699; US20150045546; US20150031134; US20150024500; US20140377868; US20140357530; US20140349400; US20140335620; US20140335063; US20140315985; US20140310830; US20140310828; US20140309487; US20140304853; US20140298547; US20140295556; US20140294773; US20140287938; US20140273234; US20140273232; US20140273231; US20140273230; US20140271987; US20140256046; US20140248702; US20140242702; US20140242700; US20140242699; US20140242664; US20140234972; US20140227787; US20140212869; US20140201857; US20140199767; US20140189896; US20140186958; US20140186919; US20140186843; US20140179770; US20140179006; US20140170753; WO/2008/108989; WO/2010/054108; WO/2012/164565; WO/2013/098244; WO/2013/176772; US 20150071899; Makarova et al., “Evolution and classification of the CRISPR-Cas systems” 9(6) Nature Reviews Microbiology 467-477 (1-23) (June 2011); Wiedenheft et al., “RNA-guided genetic silencing systems in bacteria and archaea” 482 Nature 331-338 (Feb. 16, 2012); Gasiunas et al., “Cas9-crRNA ribonucleoprotein complex mediates specific DNA cleavage for adaptive immunity in bacteria” 109(39) Proceedings of the National Academy of Sciences USA E2579-E2586 (Sep. 4, 2012); Jinek et al., “A Programmable Dual-RNA-Guided DNA Endonuclease in Adaptive Bacterial Immunity” 337 Science 816-821 (Aug. 17, 2012); Carroll, “A CRISPR Approach to Gene Targeting” 20(9) Molecular Therapy 1658-1660 (September 2012); U.S. Appl. No. 61/652,086, filed May 25, 2012; Al-Attar et al., Clustered Regularly Interspaced Short Palindromic Repeats (CRISPRs): The Hallmark of an Ingenious Antiviral Defense Mechanism in Prokaryotes, Biol Chem. (2011) vol. 392, Issue 4, pp. 277-289; Hale et al., Essential Features and Rational Design of CRISPR RNAs That Function With the Cas RAMP Module Complex to Cleave RNAs, Molecular Cell, (2012) vol. 45, Issue 3, 292-302.

The variant proteins described herein can be used in place of or in addition to any of the Cas9 proteins described in the foregoing references, or in combination with mutations described therein. In addition, the variants described herein can be used in fusion proteins in place of the wild-type Cas9 or other Cas9 mutations (such as the dCas9 or Cas9 nickase described above) as known in the art, e.g., a fusion protein with a heterologous functional domains as described in U.S. Pat. No. 8,993,233; US 20140186958; U.S. Pat. No. 9,023,649; WO/2014/099744; WO 2014/089290; WO2014/144592; WO144288; WO2014/204578; WO2014/152432; WO2115/099850; U.S. Pat. No. 8,697,359; US2010/0076057; US2011/0189776; US2011/0223638; US2013/0130248; WO/2008/108989; WO/2010/054108; WO/2012/164565; WO/2013/098244; WO/2013/176772; US20150050699; US 20150071899 and WO 2014/124284. For example, the variants, preferably comprising one or more nuclease-reducing, -altering, or -killing mutation, can be fused on the N or C terminus of the Cas9 to a transcriptional activation domain or other heterologous functional domains e.g., transcriptional repressors (e.g., KRAB, ERD, SID, and others, e.g., amino acids 473-530 of the ets2 repressor factor (ERF) repressor domain (ERD), amino acids 1-97 of the KRAB domain of KOX1, or amino acids 1-36 of the Mad mSIN3 interaction domain (SID); see Beerli et al., PNAS USA 95:14628-14633 (1998)) or silencers such as Heterochromatin Protein 1 (HP1, also known as swi6), e.g., HP1α or HP1β; proteins or peptides that could recruit long non-coding RNAs (lncRNAs) fused to a fixed RNA binding sequence such as those bound by the MS2 coat protein, endoribonuclease Csy4, or the lambda N protein; enzymes that modify the methylation state of DNA (e.g., DNA methyltransferase (DNMT) or TET proteins); or enzymes that modify histone subunits (e.g., histone acetyltransferases (HAT), histone deacetylases (HDAC), histone methyltransferases (e.g., for methylation of lysine or arginine residues) or histone demethylases (e.g., for demethylation of lysine or arginine residues)) as are known in the all can also be used. A number of sequences for such domains are known in the art, e.g., a domain that catalyzes hydroxylation of methylated cytosines in DNA. Exemplary proteins include the Ten-Eleven-Translocation (TET)1-3 family, enzymes that converts 5-methylcytosine (5-mC) to 5-hydroxymethylcytosine (5-hmC) in DNA.

Sequences for human TET1-3 are known in the art and are shown in the following table:

GenBank Accession Nos. Gene Amino Acid Nucleic Acid TET1 NP_085128.2 NM_030625.2 TET2* NP_001120680.1 (var 1) NM_001127208.2 NP_060098.3 (var 2) NM_017628.4 TET3 NP_659430.1 NM_144993.1 *Variant (1) represents the longer transcript and encodes the longer isoform (a). Variant (2) differs in the 5′ UTR and in the 3′ UTR and coding sequence compared to variant 1. The resulting isoform (b) is shorter and has a distinct C-terminus compared to isoform a.

In some embodiments, all or part of the full-length sequence of the catalytic domain can be included, e.g., a catalytic module comprising the cysteine-rich extension and the 2OGFeDO domain encoded by 7 highly conserved exons, e.g., the Tet1 catalytic domain comprising amino acids 1580-2052, Tet2 comprising amino acids 1290-1905 and Tet3 comprising amino acids 966-1678. See, e.g., FIG. 1 of Iyer et al., Cell Cycle. 2009 Jun. 1; 8(11):1698-710. Epub 2009 Jun. 27, for an alignment illustrating the key catalytic residues in all three Tet proteins, and the supplementary materials thereof (available at ftp site ftp.ncbi.nih.gov/pub/aravind/DONS/supplementary_material_DONS.html) for full length sequences (see, e.g., seq 2c); in some embodiments, the sequence includes amino acids 1418-2136 of Tet1 or the corresponding region in Tet2/3.

Other catalytic modules can be from the proteins identified in Iyer et al., 2009.

In some embodiments, the heterologous functional domain is a biological tether, and comprises all or part of (e.g., DNA binding domain from) the MS2 coat protein, endoribonuclease Csy4, or the lambda N protein. These proteins can be used to recruit RNA molecules containing a specific stem-loop structure to a locale specified by the dCas9 gRNA targeting sequences. For example, a dCas9 variant fused to MS2 coat protein, endoribonuclease Csy4, or lambda N can be used to recruit a long non-coding RNA (lncRNA) such as XIST or HOTAIR; see, e.g., Keryer-Bibens et al., Biol. Cell 100:125-138 (2008), that is linked to the Csy4, MS2 or lambda N binding sequence. Alternatively, the Csy4, MS2 or lambda N protein binding sequence can be linked to another protein, e.g., as described in Keryer-Bibens et al., supra, and the protein can be targeted to the dCas9 variant binding site using the methods and compositions described herein. In some embodiments, the Csy4 is catalytically inactive. In some embodiments, the Cas9 variant, preferably a dCas9 variant, is fused to FokI as described in U.S. Pat. No. 8,993,233; US 20140186958; U.S. Pat. No. 9,023,649; WO/2014/099744; WO2014/089290; WO2014/144592; WO144288; WO2014/204578; WO2014/152432; WO2115/099850; U.S. Pat. No. 8,697,359; US2010/0076057; US2011/0189776; US2011/0223638; US2013/0130248; WO/2008/108989; WO/2010/054108; WO/2012/164565; WO/2013/098244; WO/2013/176772; US20150050699; US 20150071899 and WO2014/204578.

In some embodiments, the fusion proteins include a linker between the dCas9 variant and the heterologous functional domains. Linkers that can be used in these fusion proteins (or between fusion proteins in a concatenated structure) can include any sequence that does not interfere with the function of the fusion proteins. In preferred embodiments, the linkers are short, e.g., 2-20 amino acids, and are typically flexible (i.e., comprising amino acids with a high degree of freedom such as glycine, alanine, and serine). In some embodiments, the linker comprises one or more units consisting of GGGS (SEQ ID NO:3) or GGGGS (SEQ ID NO:4), e.g., two, three, four, or more repeats of the GGGS (SEQ ID NO:5) or GGGGS (SEQ ID NO:6) unit. Other linker sequences can also be used.

In some embodiments, the variant protein includes a cell-penetrating peptide sequence that facilitates delivery to the intracellular space, e.g., HIV-derived TAT peptide, penetratins, transportans, or hCT derived cell-penetrating peptides, see, e.g., Caron et al., (2001) Mol Ther. 3(3):310-8; Langel, Cell-Penetrating Peptides: Processes and Applications (CRC Press, Boca Raton Fla. 2002); El-Andaloussi et al., (2005) Curr Pharm Des. 11(28):3597-611; and Deshayes et al., (2005) Cell Mol Life Sci. 62(16):1839-49.

Cell penetrating peptides (CPPs) are short peptides that facilitate the movement of a wide range of biomolecules across the cell membrane into the cytoplasm or other organelles, e.g. the mitochondria and the nucleus. Examples of molecules that can be delivered by CPPs include therapeutic drugs, plasmid DNA, oligonucleotides, siRNA, peptide-nucleic acid (PNA), proteins, peptides, nanoparticles, and liposomes, CPPs are generally 30 amino acids or less, are derived from naturally or non-naturally occurring protein or chimeric sequences, and contain either a high relative abundance of positively charged amino acids, e.g. lysine or arginine, or an alternating pattern of polar and non-polar amino acids. CPPs that are commonly used in the art include Tat (Frankel et al., (1988) Cell. 55:1189-1193, Vives et al., (1997) J. Biol. Chem. 272:16010-16017), penetratin (Derossi et al., (1994) J. Biol. Chem. 269:10444-10450), polyarginine peptide sequences (Wender et al., (2000) Proc. Natl. Acad. Sci. USA 97:13003-13008, Futaki et al., (2001) J. Biol. Chem 276:5836-5840), and transportan (Pooga et al., (1998) Nat. Biotechnol. 16:857-861).

CPPs can be linked with their cargo through covalent or non-covalent strategies. Methods for covalently joining a CPP and its cargo are known in the art, e.g. chemical cross-linking (Stetsenko et al., (2000) J. Org. Chem. 65:4900-4909, Gait et al. (2003) Cell. Mol. Life. Sci. 60:844-853) or cloning a fusion protein (Nagahara et al., (1998) Nat. Med. 4:1449-1453). Non-covalent coupling between the cargo and short amphipathic CPPs comprising polar and non-polar domains is established through electrostatic and hydrophobic interactions.

CPPs have been utilized in the art to deliver potentially therapeutic biomolecules into cells. Examples include cyclosporine linked to polyarginine for immunosuppression (Rothbard et al., (2000) Nature Medicine 6(11):1253-1257), siRNA against cyclin B1 linked to a CPP called MPG for inhibiting tumorigenesis (Crombez et al., (2007) Biochem Soc. Trans. 35:44-46), tumor suppressor p53 peptides linked to CPPs to reduce cancer cell growth (Takenobu et al., (2002) Mol. Cancer Ther. 1(12):1043-1049, Snyder et al., (2004) PLoS Biol. 2:E36), and dominant negative forms of Ras or phosphoinositol 3 kinase (PI3K) fused to Tat to treat asthma (Myou et al., (2003) J. Immunol. 171:4399-4405).

CPPs have been utilized in the art to transport contrast agents into cells for imaging and biosensing applications. For example, green fluorescent protein (GFP) attached to Tat has been used to label cancer cells (Shokolenko et al., (2005) DNA Repair 4(4):511-518). Tat conjugated to quantum dots have been used to successfully cross the blood-brain barrier for visualization of the rat brain (Santra et al., (2005) Chem. Commun. 3144-3146). CPPs have also been combined with magnetic resonance imaging techniques for cell imaging (Liu et al. (2006) Biochem. and Biophys. Res. Comm. 347(1):133-140). See also Ramsey and Flynn, Pharmacol Ther. 2015 Jul. 22. pii: S0163-7258(15)00141-2.

Alternatively, or in addition, the variant proteins can include a nuclear localization sequence, e.g., SV40 large T antigen NLS (PKKKRRV (SEQ ID NO:7)) and nucleoplasmin NLS (KRPAATKKAGQAKKKK (SEQ ID NO:8)). Other NLSs are known in the art; see, e.g., Cokol et al., EMBO Rep. 2000 Nov. 15; 1(5): 411-415; Freitas and Cunha, Curr Genomics. 2009 December; 10(8): 550-557.

In some embodiments, the variants include a moiety that has a high affinity for a ligand, for example GST, FLAG or hexahistidine sequences. Such affinity tags can facilitate the purification of recombinant variant proteins.

For methods in which the variant proteins are delivered to cells, the proteins can be produced using any method known in the art, e.g., by in vitro translation, or expression in a suitable host cell from nucleic acid encoding the variant protein; a number of methods are known in the art for producing proteins. For example, the proteins can be produced in and purified from yeast, E. coli, insect cell lines, plants, transgenic animals, or cultured mammalian cells; see, e.g., Palomares et al., “Production of Recombinant Proteins: Challenges and Solutions,” Methods Mol Biol. 2004; 267:15-52. In addition, the variant proteins can be linked to a moiety that facilitates transfer into a cell, e.g., a lipid nanoparticle, optionally with a linker that is cleaved once the protein is inside the cell. See, e.g., Lafountaine et al., Int J Pharm. 2015 Aug. 13; 494(1):180-194.

Expression Systems

To use the Cas9 variants described herein, it may be desirable to express them from a nucleic acid that encodes them. This can be performed in a variety of ways. For example, the nucleic acid encoding the Cas9 variant can be cloned into an intermediate vector for transformation into prokaryotic or eukaryotic cells for replication and/or expression. Intermediate vectors are typically prokaryote vectors, e.g., plasmids, or shuttle vectors, or insect vectors, for storage or manipulation of the nucleic acid encoding the Cas9 variant for production of the Cas9 variant. The nucleic acid encoding the Cas9 variant can also be cloned into an expression vector, for administration to a plant cell, animal cell, preferably a mammalian cell or a human cell, fungal cell, bacterial cell, or protozoan cell.

To obtain expression, a sequence encoding a Cas9 variant is typically subcloned into an expression vector that contains a promoter to direct transcription. Suitable bacterial and eukaryotic promoters are well known in the art and described, e.g., in Sambrook et al., Molecular Cloning, A Laboratory Manual (3d ed. 2001); Kriegler, Gene Transfer and Expression: A Laboratory Manual (1990); and Current Protocols in Molecular Biology (Ausubel et al., eds., 2010). Bacterial expression systems for expressing the engineered protein are available in, e.g., E. coli, Bacillus sp., and Salmonella (Palva et al., 1983, Gene 22:229-235). Kits for such expression systems are commercially available. Eukaryotic expression systems for mammalian cells, yeast, and insect cells are well known in the art and are also commercially available.

The promoter used to direct expression of a nucleic acid depends on the particular application. For example, a strong constitutive promoter is typically used for expression and purification of fusion proteins. In contrast, when the Cas9 variant is to be administered in vivo for gene regulation, either a constitutive or an inducible promoter can be used, depending on the particular use of the Cas9 variant. In addition, a preferred promoter for administration of the Cas9 variant can be a weak promoter, such as HSV TK or a promoter having similar activity. The promoter can also include elements that are responsive to transactivation, e.g., hypoxia response elements. Gal4 response elements, lac repressor response element, and small molecule control systems such as tetracycline-regulated systems and the RU-486 system (see, e.g., Gossen & Bujard, 1992, Proc. Natl. Acad. Sci. USA, 89:5547; Oligino et al., 1998, Gene Ther., 5:491-496; Wang et al., 1997, Gene Ther., 4:432-441; Neering et al., 1996, Blood, 88:1147-55; and Rendahl et al., 1998, Nat. Biotechnol., 16:757-761).

In addition to the promoter, the expression vector typically contains a transcription unit or expression cassette that contains all the additional elements required for the expression of the nucleic acid in host cells, either prokaryotic or eukaryotic. Atypical expression cassette thus contains a promoter operably linked, e.g., to the nucleic acid sequence encoding the Cas9 variant, and any signals required, e.g., for efficient polyadenylation of the transcript, transcriptional termination, ribosome binding sites, or translation termination. Additional elements of the cassette may include, e.g., enhancers, and heterologous spliced intronic signals.

The particular expression vector used to transport the genetic information into the cell is selected with regard to the intended use of the Cas9 variant, e.g., expression in plants, animals, bacteria, fungus, protozoa, etc. Standard bacterial expression vectors include plasmids such as pBR322 based plasmids, pSKF, pET23D, and commercially available tag-fusion expression systems such as GST and LacZ.

Expression vectors containing regulatory elements from eukaryotic viruses are often used in eukaryotic expression vectors, e.g., SV40 vectors, papilloma virus vectors, and vectors derived from Epstein-Barr virus. Other exemplary eukaryotic vectors include pMSG, pAV009/A+, pMTO10/A+, pMAMneo-5, baculovirus pDSVE, and any other vector allowing expression of proteins under the direction of the SV40 early promoter, SV40 late promoter, metallothionein promoter, murine mammary tumor virus promoter, Rous sarcoma virus promoter, polyhedrin promoter, or other promoters shown effective for expression in eukaryotic cells.

The vectors for expressing the Cas9variants can include RNA Pol III promoters to drive expression of the guide RNAs, e.g., the H1, U6 or 7SK promoters. These human promoters allow for expression of Cas9 variants in mammalian cells following plasmid transfection.

Some expression systems have markers for selection of stably transfected cell lines such as thymidine kinase, hygromycin B phosphotransferase, and dihydrofolate reductase. High yield expression systems are also suitable, such as using a baculovirus vector in insect cells, with the gRNA encoding sequence under the direction of the polyhedrin promoter or other strong baculovirus promoters.

The elements that are typically included in expression vectors also include a replicon that functions in E. coli, a gene encoding antibiotic resistance to permit selection of bacteria that harbor recombinant plasmids, and unique restriction sites in nonessential regions of the plasmid to allow insertion of recombinant sequences.

Standard transfection methods are used to produce bacterial, mammalian, yeast or insect cell lines that express large quantities of protein, which are then purified using standard techniques (see, e.g., Colley et al., 1989, J. Biol. Chem., 264:17619-22; Guide to Protein Purification, in Methods in Enzymology, vol. 182 (Deutscher, ed., 1990)). Transformation of eukaryotic and prokaryotic cells are performed according to standard techniques (see, e.g., Morrison, 1977, J. Bacteriol. 132:349-351; Clark-Curtiss & Curtiss, Methods in Enzymology 101:347-362 (Wu et al., eds, 1983).

Any of the known procedures for introducing foreign nucleotide sequences into host cells may be used. These include the use of calcium phosphate transfection, polybrene, protoplast fusion, electroporation, nucleofection, liposomes, microinjection, naked DNA, plasmid vectors, viral vectors, both episomal and integrative, and any of the other well-known methods for introducing cloned genomic DNA, cDNA, synthetic DNA or other foreign genetic material into a host cell (see, e.g., Sambrook et al., supra). It is only necessary that the particular genetic engineering procedure used be capable of successfully introducing at least one gene into the host cell capable of expressing the Cas9 variant.

The present methods can also include modifying gDNA by introducing purified Cas9 protein with a gRNA into cells as a ribonuclear protein (RNP) complex, as well as introducing a gRNA plus mRNA encoding the Cas9 protein. The gRNA can be synthetic gRNA or a nucleic acid (e.g., in an expression vector) encoding the guide RNA.

The present invention also includes the vectors and cells comprising the vectors.

EXAMPLES

The invention is further described in the following examples, which do not limit the scope of the invention described in the claims.

Methods

Bacterial-based Positive Selection Assay for Evolving SpCas9 Variants

Competent E. coli BW25141(λDE3)²³ containing a positive selection plasmid (with embedded target site) were transformed with Cas9/sgRNA-encoding plasmids. Following a 60-minute recovery in SOB media, transformations were plated on LB plates containing either chloramphenicol (non-selective) or chloramphenicol+10 mM arabinose (selective).

To identify additional positions that might be critical for genome wide target specificity, a bacterial selection system previously used to study properties of homing endonucleases (hereafter referred to as the positive selection) (Chen & Zhao, Nucleic Acids Res 33, e154 (2005); Doyon et al., J Am Chem Soc 128, 2477-2484 (2006)) was adapted.

In the present adaptation of this system, Cas9-mediated cleavage of a positive selection plasmid encoding an inducible toxic gene enables cell survival, due to subsequent degradation and loss of the linearized plasmid. After establishing that SpCas9 can function in the positive selection system, both wild-type and the variants were tested for their ability to cleave a selection plasmid harboring a target site selected from the known human genome. These variants were introduced into bacteria with a positive selection plasmid containing a target site and plated on selective medium. Cleavage of the positive selection plasmid was estimated by calculating the survival frequency: colonies on selective plates/colonies on non-selective plates (see FIGS. 1,5-6).

A Subset of Plasmids Used in this Study (Sequences Shown Below)

Name Addgene ID Description JDS246 43861 CMV-T7-humanSpCas9-NLS-3xFLAG VP12 pending CMV-T7-humanSpCas9-HF1(N497A, R661A, Q695A, Q926A)-NLS-3xFLAG MSP2135 pending CMV-T7-humanSpCas9-HF2(N497A, R661A, Q695A, Q926A, D1135E)- NLS-3xFLAG MSP2133 pending CMV-T7-humanSpCas9-HF4(Y450A, N497A, R661A, Q695A, Q926A)- NLS-3xFLAG MSP469 65771 CMV-T7-humanSpCas9-VQR(D1135V, R1335Q, T1337R)-NLS-3xFLAG MSP2440 pending CMV-T7-humanSpCas9-VQR-HF1(N497A, R661A, Q695A, Q926A, D1135V, R1335Q, T1337R)-NLS-3xFLAG BPK2797 pending CMV-T7-humanSpCas9-VRQR(D1135V, G1218R, R1335Q, T1337R)-NLS-3xFLAG MSP2443 pending CMV-T7-humanSpCas9-VRQR-HF1(N497A, R661A, Q695A, Q926A, D1135V, G1218R, R1335Q, T1337R)-NLS-3xFLAG BPK1520 65777 U6-BsmBIcassette-Sp-sgRNA

Human Cell Culture and Transfection

U2OS.EGFP cells harboring a single integrated copy of a constitutively expressed EGFP-PEST reporter gene¹⁵ were cultured in Advanced DMEM media (Life Technologies) supplemented with 10% FBS, 2 mM GlutaMax (Life Technologies), penicillin/streptomycin, and 400 μg/ml of G418 at 37°C. with 5% CO₂. Cells were co-transfected with 750 ng of Cas9 plasmid and 250 ng of sgRNA plasmid (unless otherwise noted) using the DN-100 program of a Lonza 4D-nucleofector according to the manufacturer's protocols. Cas9 plasmid transfected together with an empty U6 promoter plasmid was used as a negative control for all human cell experiments. (see FIGS. 2, 7-10).

Human Cell EGFP Disruption Assay

EGFP disruption experiments were performed as previously described¹⁶. Transfected cells were analyzed for EGFP expression ˜52 hours post-transfection using a Fortessa flow cytometer (BD Biosciences). Background EGFP loss was gated at approximately 2.5% for all experiments (see FIGS. 2, 7).

T7E1 Assay, Targeted Deep-sequencing, and GUIDE-seq to Quantify Nuclease-induced Mutation Rates

T7E1 assays were performed as previously described for human cells (Kleinstiver, B. P. et al., Nature 523, 481-485 (2015)). For U2OS.EGFP human cells, genomic DNA was extracted from transfected cells ˜72 hours post-transfection using the Agencourt DNAdvance Genomic DNA Isolation Kit (Beckman Coulter Genomics). Roughly 200 ng of purified PCR product was denatured, annealed, and digested with T7E1 (New England BioLabs). Mutagenesis frequencies were quantified using a Qiaxcel capillary electrophoresis instrument (QIagen), as previously described for human cells (Kleinstiver et al., Nature 523, 481-485 (2015); Reyon et al., Nat Biotechnol 30, 460-465 (2012)).

GUIDE-seq experiments were performed as previously described (Tsai et al., Nat Biotechnol 33, 187-197 (2015)). Briefly, phosphorylated, phosphorothioate-modified double-stranded oligodeoxynucleotides (dsODNs) were transfected into U2OS cells with Cas9 nuclease along with Cas9 and sgRNA expression plasmids, as described above. dsODN-specific amplification, high-throughput sequencing, and mapping were performed to identify genomic intervals containing DSB activity. For wild-type versus double or quadruple mutant variant experiments, off-target read counts were normalized to the on-target read counts to correct for sequencing depth differences between samples. The normalized ratios for wild-type and variant SpCas9 were then compared to calculate the fold-change in activity at off-target sites. To determine whether wild-type and SpCas9 variant samples for GUIDE-seq had similar oligo tag integration rates at the intended target site, restriction fragment length polymorphism (RFLP) assays were performed by amplifying the intended target loci with Phusion Hot-Start Flex from 100 ng of genomic DNA (isolated as described above). Roughly 150 ng of PCR product was digested with 20 U of Ndel (New England BioLabs) for 3 hours at 37° C. prior to clean-up using the Agencourt Ampure XP kit. RFLP results were quantified using a Qiaxcel capillary electrophoresis instrument (QIagen) to approximate oligo tag integration rates. T7E1 assays were performed for a similar purpose, as described above.

Example 1

One potential solution to address targeting specificity of CRISPR-Cas9 RNA guided gene editing would be to engineer Cas9 variants with novel mutations.

Based on these earlier results, it was hypothesized (without wishing to be bound by theory) that the specificity of CRISPR-Cas9 nucleases might be significantly increased by reducing the non-specific binding affinity of Cas9 for DNA, mediated by the binding to the phosphate groups on the DNA or hydrophobic or base stacking interactions with the DNA. This approach would have the advantage of not decreasing the length of the target site recognized by the gRNA/Cas9 complex, as in the previously described truncated gRNA approach. It was reasoned that non-specific binding affinity of Cas9 for DNA might be reduced by mutating amino acid residues that contact phosphate groups on the target DNA.

An analogous approach has been used to create variants of non-Cas9 nucleases such as TALENs (see, for example, Guilinger et al., Nat. Methods. 11: 429 (2014)).

In an initial test of the hypothesis, the present inventors attempted to engineer a reduced affinity variant of the widely used S pyogenes Cas9 (SpCas9) by introducing individual alanine substitutions into various residues in SpCas9 that might be expected to interact with phosphates on the DNA backbone. An E.coli-based screening assay was used to assess the activities of these variants (Kleinstiver et al., Nature. 2015 Jul. 23; 523(7561):481-5). In this bacterial system, cell survival depended on cleavage (and subsequent destruction) of a selection plasmid containing a gene for the toxic gyrase poison ccdB and a 23 base pair sequence targeted by a gRNA and SpCas9. Results of this experiment identified residues that retained or lost activity (Table 1).

TABLE 1 Activities of single alanine substitution mutants of Cas9 as assessed in the bacterial cell-based system shown in FIG. 1. mutation % survival R63A 84.2 R66A 0 R70A 0 R74A 0 R78A 56.4 R165A 68.9 R403A 85.2 N407A 97.2 N497A 72.6 K510A 79.0 Y515A 34.1 R661A 75.0 Q695A 69.8 Q926A 53.3 K1107A 47.4 E1108A 40.0 S1109A 96.6 K1113A 51.8 R1114A 47.3 S1116A 73.8 K1118A 48.7 D1135A 67.2 S1136A 69.2 K1151A 0 K1153A 76.6 K1155A 44.6 K1158A 46.5 K1185A 19.3 K1200A 24.5 S1216A 100.4 Q1221A 98.8 K1289A 55.2 R1298A 28.6 K1300A 59.8 K1325A 52.3 R1333A 0 K1334A 87.5 R1335A 0 T1337A 64.6 Survival percentages between 50-100% usually indicated robust cleavage, whereas 0% survival indicated that the enzyme has been functionally compromised. Additional mutations that were assayed in bacteria (but are not shown in the table above) include: R69A, R71A, Y72A, R75A, K76A, N77A, R115A, H160A, K163A, L169A, T404A, F405A, R447A, I448A, Y450A, S460A, M495A, M694A, H698A, Y1013A, V1015A, R1122A, K1123A, and K1124A. With the exception of R69A and F405A (which had <5% survival in bacteria), all of these additional single mutations appeared to have little effect on the on-target activity of SpCas9 (>70% survival in the bacterial screen).

15 different SpCas9 variants bearing all possible single, double, triple and quadruple combinations of the N497A, R661A, Q695A, and Q926A mutations were constructed to test whether contacts made by these residues might be dispensable for on-target activity (FIG. 1b ). For these experiments, a previously described human cell-based assay was used in which cleavage and induction of insertion or deletion mutations (indels) by non-homologous end-joining (NHEJ)-mediated repair within a single integrated EGFP reporter gene leads to loss of cell fluorescence (Reyon, D. et al., Nat Biotechnol. 30, 460-465, 2012). Using a EGFP-targeted sgRNA previously shown to efficiently disrupt EGFP expression in human cells when paired with wild-type SpCas9 (Fu, Y. et al., Nat Biotechnol 31, 822-826 (2013), all 15 SpCas9 variants possessed EGFP disruption activities comparable to that of wild-type SpCas9 (FIG. 1b , grey bars). Thus, substitution of one or all of these residues did not reduce on-target cleavage efficiency of SpCas9 with this EGFP-targeted sgRNA.

Next, experiments were performed to assess the relative activities of all 15 SpCas9 variants at mismatched target sites. To do this, the EGFP disruption assay was repeated with derivatives of the EGFP-targeted sgRNA used in the previous experiment that contain pairs of substituted bases at positions 13 and 14, 15 and 16, 17 and 18, and 18 and 19 (numbering starting with 1 for the most PAM-proximal base and ending with 20 for the most PAM-distal base; FIG. 1b ). This analysis revealed that one of the triple mutants (R661A/Q695A/Q926A) and the quadruple mutant (N497A/R661A/Q695A/Q926A) both showed levels of EGFP disruption equivalent to that of background with all four of the mismatched sgRNAs (FIG. 1b , colored bars). Notably, among the 15 variants, those possessing the lowest activities with the mismatched sgRNAs all harbored the Q695A and Q926A mutations. Based on these results and similar data from an experiment using a sgRNA for another EGFP target site, the quadruple mutant (N497A/R661A/Q695A/Q926A) was chosen for additional analysis and designated it as SpCas9-HF1 (for high-fidelity variant #1).

On-target Activities of SpCas9-HF1

To determine how robustly SpCas9-HF1 functions at a larger number of on-target sites, direct comparisons were performed between this variant and wild-type SpCas9 using additional sgRNAs. In total, 37 different sgRNAs were tested: 24 targeted to EGFP (assayed with the EGFP disruption assay) and 13 targeted to endogenous human gene targets (assayed using the T7 Endonuclease I (T7EI) mismatch assay). 20 of the 24 sgRNAs tested with the EGFP disruption assay (FIG. 1c ) and 12 of the 13 sgRNAs tested on endogenous human gene sites (FIG. 1d ) showed activities with SpCas9-HF1 that were at least 70% as active as wild-type SpCas9 with the same sgRNA (FIG. 1e ). Indeed, SpCas9-HF1 showed highly comparable activities (90-140%) to wild-type SpCas9 with the vast majority of sgRNAs (FIG. 1e ). Three of the 37 sgRNAs tested showed essentially no activity with SpCas9-HF1 and examination of these target sites did not suggest any obvious differences in the characteristics of these sequences compared to those for which high activities were seen (Table 3). Overall, SpCas9-HF1 possessed comparable activities (greater than 70% of wild-type SpCas9 activities) for 86% (32/37) of the sgRNAs tested.

TABLE 3 List of sgRNA targets Spacer SEQ Sequence SEQ Prep length Spacer ID with extended ID Name Name (nt) Sequence NO: PAM NO: S. pyogenes sgRNAs EGFP FYF1 NGG 20 GGGCACGGGC   9. GGGCACGGGCAGCTTGC  10. 320 site 1 AGCTTGCCGG CGGTGGT FYF1 NGG 18 GCACGGGCA  11. GCACGGGCAGCTTGCCG  12. 641 site 1 GCTTGCCGG GTGGT CK10 NGG 20 GGGCACccGC  13. GGGCACccGCAGCTTGC  14. 12 site 1- AGCTTGCCGG CGGTGGT 13 & 14 FYF1 NGG 20 GGGCtgGGGC  15. GGGCtgGGGCAGCTTGC  16. 429 site 1- AGCTTGCCGG CGGTGGT 15 & 16 FYF1 NGG 20 GGcgACGGGC  17. GGcgACGGGCAGCTTGC  18. 430 site 1- AGCTTGCCGG CGGTGGT 17 & 18 FYF1 NGG 20 GccCACGGGC  19. GccCACGGGCAGCTTGC  20. 347 site 1- AGCTTGCCGG CGGTGGT 18 & 19 BPK1 NGG 20 GTCGCCCTCG  21. GTCGCCCTCGAACTTCA  22. 345 site 2 AACTTCACCT CCTCGGC BPK1 NGG 20 GTAGGTCAGG  23. GTAGGTCAGGGTGGTCA  24. 350 site 3 GTGGTCACGA CGAGGG BPK1 NGG 20 GGCGAGGGCG  25. GGCGAGGGCGATGCCAC  26. 353 site 4 ATGCCACCTA CTACGGC MSP7 NGG 20 GGTCGCCACC  27. GGTCGCCACCATGGTGA  28. 92 site 5 ATGGTGAGCA GCAAGGC MSP7 NGG 20 GGTCAGGGTG  29. GGTCAGGGTGGTCACGA  30. 95 site 6 GTCACGAGGG GGGTGGG FYF1 NGG 20 GGTGGTGCAG  31. GGTGGTGCAGATGAACT  32. 328 site 7 ATGAACTTCA TCAGGGT JAF1 NGG 17 GGTGCAGATG  33. GGTGCAGATGAACTTCA  34. 001 site 7 AACTTCA GGGT BPK1 NGG 20 GTTGGGGTCT  35. GTTGGGGTCTTTGCTCA  36. 365 site 8 TTGCTCAGGG GGGCGGA MSP7 NGG 20 GGTGGTCACG  37. GGTGGTCACGAGGGTGG  38. 94 site 9 AGGGTGGGCC GCCAGGG FYF1 NGG 20 GATGCCGTTC  39. GATGCCGTTCTTCTGCT  40. 327 site 10 TTCTGCTTGT TGTCGGC JAF9 NGG 17 GCCGTTCTTC  41. GCCGTTCTTCTGCTTGT  42. 97 site 10 TGCTTGT CGGC BPK1 NGG 20 GTCGCCACCA  43. GTCGCCACCATGGTGAG  44. 347 site 11 TGGTGAGCAA CAAGGGC BPK1 NGG 20 GCACTGCACG  45. GCACTGCACGCCGTGGA  46. 369 site 12 CCGTAGGTCA TCAGGGT MSP2 NGG 20 GTGAACCGCA  47. GTGAACCGCATCGAGCT  48. 545 site 13 TCGAGCTGAA GAAGGGC MSP2 NGG 20 GAAGGGCATC  49. GAAGGGCATCGACTTCA  50. 546 site 14 GACTTCAAGG AGGAGGA MSP2 NGG 20 GCTTCATGTG  51. GCTTCATGTGGTCGGGG  52. 547 site 15 GTCGGGGTAG TAGCGGC MSP2 NGG 20 GCTGAAGCAC  53. GCTGAAGCACTGCACGC  54. 548 site 16 TGCACGCCGT CGTAGGT MSP2 NGG 20 GCCGTCGTCC  55. GCCGTCGTCCTTGAAGA  56. 549 site 17 TTGAAGAAGA AGATGGT MSP2 NGG 20 GACCAGGATG  57. GACCAGGATGGGCACCA  58. 550 site 18 GGCACCACCC CCCCGGT MSP2 NGG 20 GACGTAGCCT  59. GACGTAGCCTTCGGGCA  60. 551 site 19 TCGGGCATGG TGGCGGA MSP2 NGG 20 GAAGTTCGAG  61. GAAGTTCGAGGGCGACA  62. 553 site 20 GGCGACACCC CCCTGGT MSP2 NGG 20 GAGCTGGACG  63. GAGCTGGACGGCGACGT  64. 554 site 21 GCGACGTAAA AAACGGC MSP2 NGG 20 GGCATCGCCC  65. GGCATCGCCCTCGCCCT  66. 555 site 22 TCGCCCTCGC CGCCGGA MSP2 NGG 20 GGCCACAAGT  67. GGCCACAAGTTCAGCGT  68. 556 site 23 TCAGCGTGTC GTCCGGC FYF1 NGG 20 GGGCGAGGAG  69. GGGCGAGGAGCTGTTCA  70. 331 site 24 CTGTTCACCG CCGGGGT FYF1 NGG 18 GCGAGGAGCT  71. GCGAGGAGCTGTTCACC  72. 560 site 24 GTTCACCG GGGGT BPK1 NGG 20 CCTCGAACTT  73. CCTCGAACTTCACCTCG  74. 348 site 25- CACCTCGGCG GCGCGGG no 5′ G BPK1 NGG 20 GCTCGAACTT  75. GCTCGAACTTCACCTCG  76. 349 site 25- CACCTCGGCG GCGCGGG mm 5′ G BPK1 NGG 20 CAACTACAAG  77. CAACTACAAGACCCGCG  78. 351 site 26- ACCCGCGCCG CCGAGGT no 5′ G BPK1 NGG 20 GAACTACAAG  79. GAACTACAAGACCCGCG  80. 352 site 26- ACCCGCGCCG CCGAGGT mm 5′ G BPK1 NGG 20 CGCTCCTGGA  81. CGCTCCTGGACGTAGCC  82. 373 site 27- CGTAGCCTTC TTCGGGC no 5′ G BPK1 NGG 20 GGCTCCTGGA  83. CGCTCCTGGACGTAGCC  84. 375 site 27- CGTAGCCTTC TTCGGGC mm 5′ G BPK1 NGG 20 AGGGCGAGGA  85. AGGGCGAGGAGCTGTTC  86. 377 site 28- GCTGTTCACC ACCGGGG no 5′ G BPK1 NGG 20 GGGGCGAGGA  87. GGGGCGAGGAGCTGTTC  88. 361 site 28- GCTGTTCACC ACCGGGG mm 5′ G BPK1 NGAA 20 GTTCGAGGGC  89. GTTCGAGGGCGACACCC  90. 468 site 1 GACACCCTGG TGGTGAA MSP8 NGAA 20 GTTCACCAGG  91. GTTCACCAGGGTGTCGC  92. 07 site 2 GTGTCGCCCT CCTCGAA MSP1 NGAC 20 GCCCACCCTC  93. GCCCACCCTCGTGACCA  94. 70 site 1 GTGACCACCC CCCTGAC MSP7 NGAC 20 GCCCTTGCTC  95. GCCCTTGCTCACCATGG  96. 90 site 2 ACCATGGTGG TGGCGAC MSP1 NGAT 20 GTCGCCGTCC  97. GTCGCCGTCCAGCTCGA  98. 71 site 1 AGCTCGACCA CCAGGAT MSP1 NGAT 20 GTGTCCGGCG  99. GTGTCCGGCGAGGGCGA 100. 69 site 2 AGGGCGAGGG GGGCGAT MSP1 NGAG 20 GGGGTGGTGC 101. GGGGTGGTGCCCATCCT 102. 68 site 1 CCATCCTGGT GGTCGAG MSP3 NGAG 20 GCCACCATGG 103. GCCACCATGGTGAGCAA 104. 66 site 2 TGAGCAAGGG GGGCGAG Endogenous genes EMX1 FYF1 NGG 20 GAGTCCGAGC 105. GAGTCCGAGCAGAAGAA 106. 548 site 1 AGAAGAAGAA AGAAGGGC MSP8 NGG 20 GTCACCTCCA 107. GTCACCTCCAATGACTA 108. 09 site 2 ATGACTAGGG GGGTGGG VC47 NGG 20 GGGAAGACTG 109. GGGAAGACTGAGGCTAC 110. 5 site 3 AGGCTACATA ATAGGGT MSP8 NGA 20 GCCACGAAGC 111. GCCACGAAGCAGGCCAA 112. 14 *1 site 1 AGGCCAATGG TGGGGAG FANCF DR34 NGG 20 GGAATCCCTT 113. GGAATCCCTTCTGCAGC 114. 8 site 1 CTGCAGCACC ACCTGGA MSP8 NGG 20 GCTGCAGAAG 115. GCTGCAGAAGGGATTCC 116. 15 site 2 GGATTCCATG ATGAGGT MSP8 NGG 20 GGCGGCTGCA 117. GGCGGCTGCACAACCAG 118. 16 site 3 CAACCAGTGG TGGAGGC MSP8 NGG 20 GCTCCAGAGC 119. GCTCCAGAGCCGTGCGA 120. 17 site 4 CGTGCGAATG ATGGGGC MSP8 NGA 20 GAATCCCTTC 121. GAATCCCTTCTGCAGCA 122. 18 *2 site 1 TGCAGCACCT CCTGGAT MSP8 NGA 20 GCGGCGGCTG 123. GCGGCGCCTGCACAACC 124. 20 *3 site 2 CACAACCAGT AGTGGAG MSP8 NGA 20 GGTTGTGCAG 125. GGTTGTGCAGCCGCCGC 126. 85 *4 site 3 CCGCCGCTCC TCCAGAG RUNX1 MSP8 NGG 20 GCATTTTCAG 127. GCATTTTCAGGAGGAAG 128. 22 site 1 GAGGAAGCGA CGATGGC MSP8 NGG 20 GGGAGAAGAA 129. GGGAGAAGAAAGAGAGA 130. 25 site 2 AGAGAGATGT TGTAGGG MSP8 NGA 20 GGTGCATTTT 131. GGTGCATTTTCAGGAGG 132. 26 *5 site 1 CAGGAGGAAG AAGCGAT MSP8 NGA 20 GAGATGTAGG 133. GAGATGTAGGGCTAGAG 134. 28 *6 site 2 GCTAGAGGGG GGGTGAG MSP1 NGAA 20 GGTATCCAGC 135. GGTATCCAGCAGAGGGG 136. 725 site 1 AGAGGGGAGA AGAAGAA MSP1 NGAA 20 GAGGCATCTC 137. GAGGCATCTCTGCACCG 138. 726 site 2 TGCACCGAGG AGGTGAA MSP1 NGAC 20 GAGGGGTGAG 139. GAGGGGTGAGGCTGAAA 140. 728 site 1 GCTGAAACAG CAGTGAC MSP1 NGAC 20 GAGCAAAAGT 141. GAGCAAAAGTAGATATT 142. 730 site 2 AGATATTACA ACAAGAC MSP1 NGAT 20 GGAATTCAAA 143. GGAATTCAAACTGAGGC 144. 732 site 1 CTGAGGCATA ATATGAT MSP8 NGAT 20 GCAGAGGGGA 145. GCAGAGGGGAGAAGAAA 146. 29 site 2 GAAGAAAGAG GAGAGAT MSP1 NGAG 20 GCACCGAGGC 147. GCACCGAGGCATCTCTG 148. 734 site 1 ATCTCTGCAC CACCGAG MSP8 NGAG 20 GAGATGTAGG 149. GAGATGTAGGGCTAGAG 150. 28 site 2 GCTAGAGGGG GGGTGAG ZSCAN2 NN67 NGG 20 GTGCGGCAAG 151. GTGCGGCAAGAGCTTCA 152. 5 site AGCTTCAGCC GCCGGGG VEGFA VC29 NGG 20 GGGTGGGGGG 153. GGGTGGGGGGAGTTTGC 154. 7 site 1 AGTTTGCTCC TCCTGGA VC29 NGG 20 GACCCCCTCC 155. GACCCCCTCCACCCCGC 156. 9 site 2 ACCCCGCCTC CTCCGGG VC22 NGG 20 GGTGAGTGAG 157. GGTGAGTGAGTGTGTGC 158. 8 site 3 TGTGTGCGTG GTGTGGG BPK1 NGA 20 GCGAGCAGCG 159. GCGAGCAGCGTCTTCGA 160. 846 *7 site 1 TCTTCGAGAG GAGTGAG ZNF629 NN67 NGA 20 GTGCGGCAAG 161. GTGCGGCAAGAGCTTCA 162. 5 *8 site AGCTTCAGCC GCCAGAG *1, NGA EMX1 site 4 from Kleinstiver et al., Nature 2015 *2, NGA FANCF site 1 from Kleinstiver et al., Nature 2015 *3, NGA FANCF site 3 from Kleinstiver et al., Nature 2015 *4, NGA FANCF site 4 from Kleinstiver et al., Nature 2015 *5, NGA RUNX1 site 1 from Kleinstiver et al., Nature 2015 *6, NGA RUNX1 site 3 from Kleinstiver et al., Nature 2015 *7, NGA VEGFA site 1 from Kleinstiver et al., Nature 2015 *8, NGA ZNF629 site from Kleinstiver et al., Nature 2015 Geonome-wide Specificity of SpCas9-HF1

To test whether SpCas9-HF1 exhibited reduced off-target effects in human cells, the genome-wide unbiased identification of double-stranded breaks enabled by sequencing (GUIDE-seq) method was used. GUIDE-seq uses integration of a short double-stranded oligodeoxynucleotide (dsODN) tag into double-strand breaks to enable amplification and sequencing of adjacent genomic sequence, with the number of tag integrations at any given site providing a quantitative measure of cleavage efficiency (Tsai, S. Q. et al, Nat Biotechnol 33, 187-197 (2015)). GUIDE-seq was used to compare the spectrum of off-target effects induced by wild-type SpCas9 and SpCas9-HF1 using eight different sgRNAs targeted to various sites in the endogenous human EMX1, FANCF, RUNX1, and ZSCAN2 genes. The sequences targeted by these sgRNAs are unique and have variable numbers of predicted mismatched sites in the reference human genome (Table 2). Assessment of on-target dsODN tag integration (by restriction fragment length polymorphism (RFLP) assay) and indel formation (by T7EI assay) for the eight sgRNAs revealed comparable on-target activities with wild-type SpCas9 and SpCas9-HF1 (FIGS. 7a and 7b , respectively). GUIDE-seq experiments showed that seven of the eight sgRNAs induced cleavage at multiple genome-wide off-target sites (ranging from 2 to 25 per sgRNA) with wild-type SpCas9, whereas the eighth sgRNA (for FANCF site 4) did not produce any detectable off-target sites (FIGS. 2a and 2b ). However, six of the seven sgRNAs that induced indels with wild-type SpCas9 showed a strikingly complete absence of GUIDE-seq detectable off-target events with SpCas9-HF1 (FIGS. 2a and 2b ); and the remaining seventh sgRNA (for FANCF site 2) induced only a single detectable genome-wide off-target cleavage event, at a site harboring one mismatch within the protospacer seed sequence (FIG. 2a ). Collectively, the off-target sites that were not detected when using SpCas9-HF1 harbored one to six mismatches in the protospacer and/or PAM sequence (FIG. 2c ). As with wild-type SpCas9, the eighth sgRNA (for FANCF site 4) did not yield any detectable off-target cleavage events when tested with SpCas9-HF1(FIG. 2a ).

To confirm the GUIDE-seq findings, targeted amplicon sequencing was used to more directly measure the frequencies of NHEJ-mediated indel mutations induced by wild-type SpCas9 and SpCas9-HF1. For these experiments, human cells were transfected only with sgRNA- and Cas9-encoding plasmids (i.e., without the GUIDE-seq tag). Next-generation sequencing was then used to examine 36 of the 40 off-target sites that had been identified with wild-type SpCas9 for six sgRNAs in the GUIDE-seq experiments (four of the 40 sites could not be examined because they could not be specifically amplified from genomic DNA). These deep sequencing experiments showed that: (1) wild-type SpCas9 and SpCas9-HF1 induced comparable frequencies of indels at each of the six sgRNA on-target sites (FIGS. 3a and 3b ); (2) wild-type SpCas9, as expected showed statistically significant evidence of indel mutations at 35 of the 36 off-target sites (FIG. 3b ) at frequencies that correlated well with GUIDE-seq read counts for these same sites (FIGS. 3c ); and (3) the frequencies of indels induced by SpCas9-HF1 at 34 of the 36 off-target sites were indistinguishable from the background level of indels observed in samples from control transfections (FIG. 3b ). For the two off-target sites that appeared to have statistically significant mutation frequencies with SpCas9-HF1 relative to the negative control, the mean frequencies of indels were 0.049% and 0.037%, levels at which it is difficult to determine whether these are due to sequencing/PCR error or are bona fide nuclease-induced indels. Based on these results, it was concluded that SpCas9-HF1 can completely or nearly completely reduce off-target mutations that occur across a range of different frequencies with wild-type SpCas9 to undetectable levels.

Next the capability of SpCas9-HF1 to reduce genome-wide off-target effects of sgRNAs that target atypical homopolymeric or repetitive sequences was assessed. Although many now try to avoid on-target sites with these characteristics due to their relative lack of orthogonality to the genome, it was desirable to explore whether SpCas9-HF1 might reduce off-target indels even for these challenging targets. Therefore, previously characterized sgRNAs (Fu, Y. et al., Nat Biotechnol31, Tsai, S. Q. et al., Nat Biotechnol 33, 187-197 (2015) were used that target either a cytosine-rich homopolymeric sequence or a sequence containing multiple TG repeats in the human VEGFA gene (VEGFA site 2 and VEGFA site 3, respectively) (Table 2). In control experiments, each of these sgRNAs induced comparable levels of GUIDE-seq ds ODN tag incorporation (FIG. 7c ) and indel mutations (FIG. 7d ) with both wild-type SpCas9 and SpCas9-HF1, demonstrating that SpCas9-HF1 was not impaired in on-target activity with either of these saRNAs. Importantly, GUIDE-seq experiments revealed that SpCas9-HF1 was highly effective at reducing off-target sites of these sgRNAs, with 123/144 sites for VEGFA site 2 and 31/32 sites for VEGFA site 3 not detected (FIGS. 4a and 4b ). Examination of these off-target sites not detected with SpCas9-HF1 showed that they each possessed a range of total mismatches within their protospacer and PAM sequences: 2 to 7 mismatches for the VEGFA site 2 sgRNA and 1 to 4 mismatches for the VEGFA site 3 sgRNA (FIG. 4c ); also, nine of these off-targets for VEGFA site 2 may have a potential bulged base (Lin, Y. et al., Nucleic Acids Res 42, 7473-7485 (2014). at the sgRNA-DNA interface (FIG. 4a and FIG. 8). The sites that were not detected with SpCas9-HF1 possessed 2 to 6 mismatches for the VEGFA site 2 sgRNA and 2 mismatches in the single site for the VEGFA site 3 sgRNA (FIG. 4c ), with three off-target sites for VEGFA site 2 sgRNA again having a potential bulge (FIG. 8). Collectively, these results demonstrated that SpCas9-HF1 can be highly effective at reducing off-target effects of sgRNAs targeted to sitnple repeat sequences and can also have substantial impacts on sgRNAs targeted to homopolymeric sequences.

TABLE 21 Summary of potential mismatched sites in the reference human genome for the ten sgRNAs examined by GUIDE-seq mismatches to on-target site* site spacer with PAM 1 2 3 4 5 6 total EMX1-1 GAGTCCGAGCAGAAGAAGAAGGG 0  1  18  273  2318 15831 18441 (SEQ ID NO: 163) EMX1-2 GTCACCTCCAATGACTAGGGTGG 0  0   3   68   780  6102  6953 (SEQ ID NO: 164) FANCF-1 GGAATCCCTTCTGCAGCACCTGG 0  1  18  288  1475  9611 11393 (SEQ ID NO: 165) FANCF-2 GCTGCAGAAGGGATTCCATGAGG 1  1  29  235  2000 13047 15313 (SEQ ID NO: 166) FANCF-3 GGCGGCTGCACAACCAGTGGAGG 0  0  11   79   874  6651  7615 (SEQ ID NO: 167) FANCF-4 GCTCCAGAGCCGTGCGAATGGGG 0  0   6   59   639  5078  5782 (SEQ ID NO: 168) RUNX1-1 GCATTTTCAGGAGGAAGCGATGG 0  2   6  189  1644 11546 13387 (SEQ ID NO: 169) ZSCAN2 GTGCGGCAAGAGCTTCAGCCGGG 0  3  12  127  1146 10687 11975 (SEQ ID NO: 170) VEGFA2 GACCCCCTCCACCCCGCCTCCGG 0  2  35  456  3905 17576 21974 (SEQ ID NO: 171) VEGFA3 GGTGAGTGAGTGTGTGCGTGTGG 1 17 383 6089 13536 35901 55927 (SEQ ID NO: 172) *determined using Cas-OFFinder (Bae et al., Bioinfomatics 30, 1473-1475 (2014))

TABLE 4 Oligonucleotides used in the study SEQ ID description of T7E1 primers sequence NO: forward primer to amplify EMX1  GGAGCAGCTGGTCAG 173. in U2OS human cells AGGGG reverse primer to amplify EMX1  CCATAGGGAAGGGGG 174. in U2OS human cells ACACTGG forward primer to amplify FANCF  GGGCCGGGAAAGAGT 175. in U2OS human cells TGCTG reverse primer to amplify FANCF  GCCCTACATCTGCTCT 176. in U2OS human cells CCCTCC forward primer to amplify RUNX1  CCAGCACAACTTACTC 177. in U2OS human cells GCACTTGAC reverse primer to amplify RUNX1  CATCACCAACCCACAG 178. in U2OS human cells CCAAGG forward primer to amplify VEGFA  TCCAGATGGCACATTG 179. in U2OS human cells TCAG reverse primer to amplify VEGFA  AGGGAGCAGGAAAGT 180. in U2OS human cells GAGGT forward primer to amplify VEGFA  CGAGGAAGAGAGAGA 181. (NGG site 2) in U2OS human cells CGGGGTC reverse primer to amplify VEGFA  CTCCAATGCACCCAAG 182. (NGG site 2) in U2OS human cells ACAGCAG forward primer to amplify ZSCAN2  AGTGTGGGGTGTGTGG 183. in U2OS human cells GAAG reverse primer to amplify ZSCAN2  GCAAGGGGAAGACTC 184. in U2OS human cells TGGCA forward primer to amplify ZNF629  TACGAGTGCCTAGAGT 185. in U2OS human cells GCG reverse primer to amplify ZNF629  GCAGATGTAGGTCTTG 186. in U2OS human cells GAGGAC SEQ ID description of deep sequencing primers sequence NO: forward primer to amplify EMX1-1  GGAGCAGCTGCTCAG 187. on-target AGGGG reverse primer to amplify EMX1-1  CGATGTCCTCCCCATT 188. on-target GGCCTG forward primer to amplify EMX1-1- GTGGGGAGATTTGCAT 189. GUIDE_seq-OT#1 CTGTGGAGG reverse primer to amplify EMX1-1- GCTTTTATACCATCTT 190. GUIDE_seq-OT#1 GGGGTTACAG forward primer to amplify EMX1-1- CAATGTGCTTCAACCC 191. GUIDE_seq-OT#2 ATCACGGC reverse primer to amplify EMX1-1- CCATGAATTTGTGATG 192. GUIDE_seq-OT#2 GATGCAGTCTG forward primer to amplify EMX1-1- GAGAAGGAGGTGCAG 193. GUIDE_seq-OT#3 GAGCTAGAC reverse primer to amplify EMX1-1- CATCCCGACCTTCATC 194. GUIDE_seq-OT#3 CCTCCTGG forward primer to amplify EMX1-1- GTAGTTCTGACATTCC 195. GUIDE_seq-OT#4 TCCTGAGGG reverse primer to amplify EMX1-1- TCAAACAAGGTGCAG 196. GUIDE_seq-OT#4 ATACAGCA forward primer to amplify EMX1-1- CAGGGTCGCTCAGICT 197. GUIDE_seq-OT#5 GTGTGG reverse primer to amplify EMX1-1- CCAGCGCACCATTCAC 198. GUIDE_seq-OT#5 TCCACCTG forward primer to amplify EMX1-1- GGCTGAAGAGGAAGA 199. GUIDE_seq-OT#6 CCAGACTCAG reverse primer to amplify EMX1-1- GGCCCCTCTGAATTCA 200. GUIDE_seq-OT#6 ATTCTCTGC forward primer to amplify EMX1-1- CCACAGCGAGGAGTG 201. GUIDE_seq-OT#7 ACAGCC reverse primer to amplify EMX1-1- CCAAGTCTTTCCTAAC 202. GUIDE_seq-OT#7 TCGACCTTGG forward primer to amplify EMX1-1- CCCTAGGCCCACACCA 203. GUIDE_seq-OT#8 GCAATG reverse primer to amplify EMX1-1- GGGATGGGAATGGGA 204. GUIDE_seq-OT#8 ATGTGAGGC forward primer to amplify EMX1-2  GCCCAGGTGAAGGTGT 205. on-target GGTTCC reverse primer to amplify EMX1-2  CCAAAGCCTGGCCAGG 206. on-target GAGTG forward primer to amplify EMX1-2- AGGCAAAGATCTAGG 207. GUIDE_seq-OT#1 ACCTGGATGG reverse primer to amplify EMX1-2- CCATCTGAGTCAGCCA 208. GUIDE_seq-OT#1 GCCTTGTC forward primer to amplify EMX1-2- GGTTCCCTCCCTTCTG 209. GUIDE_seq-OT#2 AGCCC reverse primer to amplify EMX1-2- GGATAGGAATGAAGA 210. GUIDE_seq-OT#2 CCCCCTCTCC forward primer to amplify EMX1 -2- GGACTGGCTGGCTGTG 211. GUIDE_seq-OT#3 TGTTTTGAG reverse primer to amplify EMX1-2- CTTATCCAGGGCTACC 212, GUIDE_seq-OT#3 TCATTGCC forward primer to amplify EMX1-2- GCTGCTGCTGCTTTGA 213. GUIDE_seq-OT#4 TCACTCCTG reverse primer to amplify EMX1-2- CTCCTTAAACCCTCAG 214. GUIDE_seq-OT#4 AAGCTGGC forward primer to amplify EMX1-2- GCACTGTCAGCTGATC 215. GUIDE_seq-OT#5 CTACAGG reverse primer to amplify EMX1-2- ACGTTGGAACAGTCGA 216. GUIDE_seq-OT#5 GCTGTAGC forward primer to amplify EMX1-2- TGTGCATAACTCATGT 217. GUIDE_seq-OT#6 TGGCAAACT reverse primer to amplify EMX1-2- TCCACAACTACCCTCA 218. GUIDE_seq-OT#6 GCTGGAG forward primer to amplify EMX1-2- CCACTGACAATTCACT 219. GUIDE_seq-OT#7 CAACCCTGC reverse primer to amplify EMX1-2- AGGCAGACCAGTTATT 220. GUIDE_seq-OT#7 TGGCAGTC forward primer to amplify EMX1-2- ACAGGCGCAGTTCACT 221. GUIDE_seq-OT#9 GAGAAG reverse primer to amplify EMX1-2- GGGTAGGCTGACTITG 222. GUIDE_seq-OT#9 GGCTCC forward primer to amplify FANCF-1  GCCCTCTTGCCTCCAC 223. on-target TGGTTG reverse primer to amplify FANCF-1  CGCGGATGTTCCAATC 224. on-target AGTACGC forward primer to amplify FANCF-1- GCGGGCAGTGGCGTCT 225. GUIDE_seq-OT#1 TAGTCG reverse primer to amplify FANCF-1- CCCTGGGTTTGGTTGG 226. GUIDE_seq-OT#1 CTGCTC forward primer to amplify FANCF-1- CTCCTTGCCGCCCAGC 227. GUIDE_seq-OT#2 CGGTC reverse primer to amplify FANCF-1- CACTGGGGAAGAGGC 228. GUIDE_seq-OT#2 GAGGACAC forward primer to amplify FANCF-1- CCAGTGTTTCCCATCC 229. GUIDE_seq-OT#3 CCAACAC reverse primer to amplify FANCF-1- GAATGGATCCCCCCCT 230. GUIDE_seq-OT#3 AGAGCTC forward primer to amplify FANCF-1- CAGGCCCACAGGTCCT 231. GUIDE_seq-OT#4 TCTGGA reverse primer to amplify FANCF-1- CCACACGGAAGGCTG 232. GUIDE_seq-OT#4 ACCACG forward primer to amplify FANCF-3  GCGCAGAGAGAGCAG 233. on-target GACGTC reverse primer to amplify FANCF-3  GCACCTCATGGAATCC 234. on-target CTTCTGC forward primer to amplify FANCF-3- CAAGTGATGCGACTTC 235. GUIDE_seq-OT#1 CAACCTC reverse primer to amplify FANCF-3- CCCTCAGAGTTCAGCT 236. GUIDE_seq-OT#1 TAAAAAGACC forward primer to amplify FANCF-3- TGCTTCTCATCCACTCT 237. GUIDE_seq-OT#2 AGACTGCT reverse primer to amplify FANCF-3- CACCAACCAGCCATGT 238. GUIDE_seq-OT#2 GCCATG forward primer to amplify FANCF-3- CTGCCTGTGCTCCTCG 239. GUIDE_seq-OT#3 ATGGTG reverse primer to amplify FANCF-3- GGGTTCAAAGCTCATC 240. GUIDE_seq-OT#3 TGCCCC forward primer to amplify FANCF-3- GCATGTGCCTTGAGAT 241. GUIDE_seq-OT#4 TGCCTGG reverse primer to amplify FANCF-3- GACATTCAGAGAAGC 242. GUIDE_seq-OT#4 GACCATGTGG forward primer to amplify FANCF-3- CCATCTTCCCCTTTGG 243. GUIDE_seq-OT#5 CCCACAG reverse primer to amplify FANCF-3- CCCCAAAAGTGGCCAA 244. GUIDE_seq-OT#5 GAGCCTGAG forward primer to amplify FANCF-3- GTTCTCCAAAGGAAGA 245. GUIDE_seq-OT#6 GAGGGGAATG reverse primer to amplify FANCF-3- GGTGCTGTGTCCTCAT 246. GUIDE_seq-OT#6 GCATCC forward primer to amplify FANCF-3- CGGCTTGCCTAGGGTC 247. GUIDE_seq-OT#7 GTTGAG reverse primer to amplify FANCF-3- CCTTCAGGGGCTCTTC 248. GUIDE_seq-OT#7 CAGGTC forward primer to amplify RUNX1-1  GGGAACTGGCAGGCA 249. on-target CCGAGG reverse primer to amplify RUNX1-1  GGGTGAGGCTGAAAC 250. on-target AGTGACC forward primer to amplify RUNX1-1- GGGAGGATGTTGGTTT 251. GUIDE_seq-OT#1 TAGGGAACTG reverse primer to amplify RUNX1-1- TCCAATCACTACATGC 252. GUIDE_seq-OT#1 CATTTTGAAGA forward primer to amplify RUNX1-1- CCACCCTCTTCCTTTG 253. GUIDE_seq-OT#2 ATCCTCCC reverse primer to amplify RUNX1-1 - TCCTCCCTACTCCTTCA 254. GUIDE_seq-OT#2 CCCAGG forward primer to amplify ZSCAN2  GAGTGCCTGACATGTG 255. on-target GGGAGAG reverse primer to amplify ZSCAN2  TCCAGCTAAAGCCTTT 256. on-target CCCACAC forward primer to amplify ZSCAN2- GAACTCTCTGATGCAC 257. GUIDE_seq-OT#1 CTGAAGGCTG reverse primer to amplify ZSCAN2- ACCGTATCAGTGTGAT 258. GUIDE_seq-OT#1 GCATGTGGT forward primer to amplify ZSCAN2- TGGGTTTAATCATGTG 259. GUIDE_seq-OT#2 TTCTGCACTATG reverse primer to amplify ZSCAN2- CCCATCTTCCATTCTG 260. GUIDE_seq-OT#2 CCCTCCAC forward primer to amplify ZSCAN2- CAGCTAGTCCATTTGT 261. GUIDE_seq-OT#3 TCTCAGACTGTG reverse primer to amplify ZSCAN2- GGCCAACATTGTGAAA 262. GUIDE_seq-OT#3 CCCTGTCTC forward primer to amplify ZSCAN2- CCAGGGACCTGTGCTT 263. GUIDE_seq-OT#4 GGGTTC reverse primer to amplify ZSCAN2- CACCCCATGACCTGGC 264. GUIDE_seq-OT#4 ACAAGTG forward primer to amplify ZSCAN2- AAGTGTTCCTCAGAAT 265. GUIDE_seq-OT#5 GCCAGCCC reverse primer to amplify ZSCAN2- CAGGAGTGCAGTTGTG 266. GUIDE_seq-OT#5 TTGGGAG forward primer to amplify ZSCAN2- CTGATGAAGCACCAGA 267. GUIDE_seq-OT#6 GAACCCACC reverse primer to amplify ZSCAN2- CACACCTGGCACCCAT 268. GUIDE_seq-OT#6 ATGGC forward primer to amplify ZSCAN2- GATCCACACTGGTGAG 269. GUIDE_seq-OT#7 AAGCCTTAC reverse primer to amplify ZSCAN2- CTTCCCACACTCACAG 270. GUIDE_seq-OT#7 CAGATGTAGG

Refining the Specificity of SpCas9-HF1

Previously described methods such as truncated gRNAs (Fu, Y. et al., Nat Biotechnol 32, 279-284 (2014)) and the SpCas9-D1135E variant (Kleinstiver, B. P. et al., Nature 523, 481-485 (2015)) can partially reduce SpCas9 off-target effects, and the present inventors wondered whether these might be combined with SpCas9-HF1 to further improve its genome-wide specificity. Testing of SpCas9-HF1 with matched full-length and truncated sgRNAs targeted to four sites in the human cell-based EGFP disruption assay revealed that shortening sgRNA complementarity length substantially impaired on-target activities (FIG. 9). By contrast, SpCas9-HF1 with an additional D1135E mutation (a variant referred to herein as SpCas9-HF2) retained 70% or more activity of wild-type SpCas9 with six of eight sgRNAs tested using a human cell-based EGFP disruption assay (FIGS. 5a and 5b ). SpCas9-HF3 and SpCas9-HF4 variants were also created harboring L169A or Y450A mutations, respectively, at positions whose side chains mediated hydrophobic non-specific interactions with the target DNA on its PAM proximal end (Nishimasu, H. et al., Cell 156, 935-949 (2014); Jiang, F., et al., Science 348, 1477-1481 (2015)). SpCas9-HF3 and SpCas9-HF4 retained 70% or more of the activities observed with wild-type SpCas9 with the same six out of eight EGFP-targeted sgRNAs (FIGS. 5a and 5b ).

To determine whether SpCas9-HF2, -HF3, and -HF4 could reduce indel frequencies at two off-target sites for the FANCF site 2 and VEGFA site 3 sgRNAs) that were resistant to SpCas9-HF1, further experiments were performed. For the FANCF site 2 off-target, which bears a single mismatch in the seed sequence of the protospacer, SpCas9-HF4 reduced indel mutation frequencies to near background level as judged by T7EI assay while also beneficially increasing on-target activity (FIG. 5c ), resulting in the greatest increase in specificity among the three variants (FIG. 5d ). For the VEGFA site 3 off-target site, which bears two protospacer mismatches (one in the seed sequence and one at the nucleotide most distal from the PAM sequence), SpCas9-HF2 showed the greatest reduction in indel formation while showing only modest effects on on-target mutation efficiency (FIG. 5c ), leading to the greatest increase in specificity among the three variants tested (FIG. 5d ). Taken together, these results demonstrate the potential for reducing off-target effects that are resistant to SpCas944F1 by introducing additional mutations at other residues that mediate non-specific DNA contacts or that may alter PAM recognition.

To generalize the T7E1 assay findings described above that show SpCas9-HF4 and SpCas9-HF2 have improved discrimination relative to SpCas9-HF1 against off-targets of the FANCF site 2 and VEGFA site 3 sgRNAs, respectively, the genome-wide specificities of these variants were examined using GUIDE-seq. Using an RFLP assay, it was determined that SpCas9-HF4 and SpCas9-HF2 had similar on-target activities to SpCas9-HF1, as assayed by GUIDE-seq tag integration rates (FIG. 5E). When analyzing the GUIDE-seq data, no new off-target sites were identified for SpCas9-HF2 or SpCas9-HF4 (FIG. 5F), Compared to SpCas9-HF1, off-target activities at all sites were either rendered undetectable by GUIDE-seq or substantially decreased. Relative to SpCas9-HF1, SpCas9-HF4 had nearly 26-fold better specificity against the single FANCF site 2 off-target site that remained recalcitrant to the specificity improvements of SpCas9-HF1 (FIG. 5F). SpCas9-HF2 had nearly 4-fold improved specificity relative to SpCas9-HF1 for the high-frequency VEGFA site 3 off-target, while also dramatically reducing (>38-fold) or eliminating GUIDE-seq detectable events at other low-frequency off-target sites. Of note, the genomic position of 3 of these low frequency sites identified for SpCas9-HF1 are adjacent to previously characterized background U2OS cell breakpoint hotspots. Collectively, these results suggest that the SpCas9-HF2 and SpCas9-HF4 variants can improve the genome-wide specificity of SpCas9-HF1.

SpCas9-HF1 robustly and consistently reduced off-target mutations when using sgRNAs designed against standard, non-repetitive target sequences. The two off-target sites that were most resistant to SpCas9-HF1 have only one and two mismatches in the protospacer. Together, these observations suggest that off-target mutations might be minimized to undetectable levels by using SpCas9-HF1 and targeting non-repetitive sequences that do not have closely related sites bearing one or two mismatches elsewhere in the genome (something that can be easily accomplished using existing publicly available software programs (Bae, S., et al, Bioinformatics 30, 1473-1475 (2014)). One parameter that users should keep in mind is that SpCas9-HF1 may not be compatible with the common practice of using a G at the 5′ end of the gRNA that is mismatched to the protospacer sequence. Testing of four sgRNAs bearing a 5′ G mismatched to its target site showed three of the four had diminished activities with SpCas9-HF1 compared to wild-type SpCas9 (FIG. 10), perhaps reflecting the ability of SpCas9-HF1 to better discriminate a partially matched site.

Further biochemical work can confirm or clarify the precise mechanism by which SpCas9-HF₁ achieves its high genome-wide specificity. It does not appear that the four mutations introduced alter the stability or steady-state expression level of SpCas9 in the cell, because titration experiments with decreasing concentrations of expression plasmids suggested that wild-type SpCas9 and SpCas9-HF1 behaved comparably as their concentrations are lowered (FIG. 11). Instead, the simplest mechanistic explanation is that these mutations decreased the energetics of interaction between the Cas9-sgRNA and the target DNA, with the energy of the complex at a level just sufficient to retain on-target activity but lowered it enough to make off-target site cleavage inefficient or non-existent. This mechanism is consistent with the non-specific interactions observed between the residues mutated and the target DNA phosphate backbone in structural data (Nishimasu, H. et al., Cell 156, 935-949 (2014); Anders, C et. Al., Nature 513, 569-573 (2014)). A somewhat similar mechanism has been proposed to explain the increased specificities of transcription activator-like effector nucleases bearing substitutions at positively charged residues (Guilinger, J. P. et al., Nat Methods 11, 429-435 (2014)).

It was possible that SpCas9-HF1 might also be combined with other mutations that have been shown to alter Cas9 function For example, an SpCas9 mutant bearing three amino acid substitutions (D1135V/R1335Q/T1337R, also known as the SpCas9-VQR variant), recognizes sites with NGAN PAMs (with relative efficiencies for NGAG>NGAT=NGAA>NGAC) (Kleinstiver, B. P. et al, Nature 523, 481-485 (2015)) and a recently identified quadruple SpCas9 mutant (D1135V/G1218R/R1335Q/T1337R, referred to as the SpCas9-VRQR variant) has improved activities relative to the VQR variant on sites with NGAH (H=A, C, or T) PAMs (FIG. 12a ). Introduction of the four mutations (N497A/R661A/Q695A/Q926A) from SpCas9-HF1into SpCas9-VQR and SpCas9-VRQR created SpCas9-VQR-HF1 and SpCas9-VRQR-HF1, respectively. Both HF versions of these nucleases showed on-target activities comparable (i.e., 70% or more) to their non-HF counterparts with five of eight sgRNAs targeted to the EGFP reporter gene and with seven of eight sgRNAs targeted to endogenous human gene sites (FIGS. 12b-12d ).

More broadly, these results illuminate a general strategy for the engineering of additional high-fidelity variants of CRISPR-associated nucleases. Adding additional mutations at non-specific DNA contacting residues futher reduced some of the very small number of residual off-target sites that persist with SpCas9-HF1. Thus, variants such as SpCas9-HF2, SpCas9-HF3, SpCas9-HF4, and others can be utilized in a customized fashion depending on the nature of the off-target sequences. Furthermore, success with engineering high-fidelity variants of SpCas9 suggests that the approach of mutating non-specific DNA contacts can be extended to other naturally occurring and engineered Cas9 orthologues (Ran, F. A. et al., Nature 520, 186-191 (2015), Esvelt, K. M. et al., Nat Methods 10, 1116-1121 (2013); Hou, Z. et al., Proc Natl Acad Sci USA (2013); Fonfara, I. et al., Nucleic Acids Res 42, 2577-2590 (2014); Kleinstiver, B. P. et al, Nat Biotechnol (2015) as well as newer CRISPR-associated nucleases (Zetsche, B. et al., Cell 163, 759-771 (2015); Sinnakov, S. et al., Molecular Cell 60, 385-397) that are being discovered and characterized with increasing frequency.

Example 2

Described herein are SpCas9 variants with alanine substitutions in residues that contact the target strand DNA, including. N497A, Q695A, R661A, and Q926A. Beyond these residues, the present inventors sought to determine whether the specificity of these variants, e.g., the SpCas9-HF1 variant (N497A/R661A/Q695A/Q926A), might be further improved by adding substitutions in positively-charged SpCas9 residues that appear to make contacts with the non-target DNA strand: R780, K810, K832, K848, K855, K968, R976, H982, K1003, K1014, K1047, and/or R1060 (see Slaymaker et al., Science. 2016 Jan. 1; 351(6268):84-8).

The activities of wild-type SpCas9 derivatives bearing single alanine substitutions at these positions and combinations thereof were initially tested using the EGFP disruption assay with a perfectly matched sgRNA designed to a site in the EGFP gene (to assess on-target activities) and the same sgRNA bearing intentional mismatches at positions 11 and 12 with position 1 being the most PAM-proximal base (to assess activities at mismatched sites, as would be found at off-target sites) (FIG. 13A). (Note that the derivatives bearing the triple substitutions K810A/K1003A/R1060A or K848A/K1003A/R1060A are the same as recently described variants known as eSpCas9(1.0) and eSpCas9(1.1), respectively; see ref. 1). As expected, wild-type SpCas9 had robust on-target and mismatched-target activities. As a control, we also tested SpCas9-HF1 in this experiment and found that it maintained on-target activity while reducing mismatched-target activity as expected (FIG. 13A). All of the wild-type SpCas9 derivatives bearing one or more alanine substitutions at positions that might potentially contact the non-target DNA strand showed on-target activities comparable to wild-type SpCas9 (FIG. 13A). Interestingly, some of these derivatives also showed reduced cleavage with the mismatched 11/12 sgRNA relative to the activity observed with wild-type SpCas9, suggesting that a subset of the substitutions in these derivatives confer enhanced specificity against this mismatched site relative to wild-type SpCas9 (FIG. 13A). However, none of these single substitutions or combinations of substitutions were sufficient to completely eliminate activities observed the 11/12 mismatched sgRNA. When we tested wild-type SpCas9, SpCas9-HF1, and these same wild-type SpCas9 derivatives using an additional sgRNA bearing mismatches at positions 9 and 10 (FIG. 13B), only minimal changes in mismatched-target activities were observed for most derivatives. Again, this demonstrated that single, double, or even triple substitutions (equivalent to the previously described eSpCas9(1.0) and (1.1) variants) at these potential non-target strand contacting residues are insufficient to eliminate activities at imperfectly matched DNA sites. Collectively, these data demonstrate that the wild-type SpCas9 variants retain on-target activity with a matched sgRNA and that the substitutions contained in these derivatives on their own (in the context of wild-type SpCas9) are not sufficient to eliminate nuclease activities on two different mismatched DNA sites (FIGS. 13A and 13B).

Given these results, it was hypothesized that SpCas9-HF1 derivatives bearing one or more additional amino acid substitutions at residues that might contact the non-target DNA strand might further improve specificity relative to the parental SpCas9-HF1 protein. Therefore, various SpCas9-HF1-derviatives bearing combinations of single, double, or triple alanine substitutions were tested in the human cell-based EGFP disruption assay using a perfectly matched sgRNA (to test on-target activities) and the same sgRNA bearing mismatches at positions 11 and 12 (to assess activities at a mismatched target site, as would be found for off-target sites). These sgRNAs are the same ones that were used for FIGS. 13A-B. This experiment revealed most of the SpCas9-HF1-derivative variants we tested showed comparable on-target activities to those observed with both wild-type SpCas9 and SpCas9-HF1 (FIG. 14A). With the 11/12 mismatched sgRNA, some of the SpCas9-HF1 derivatives tested (such as SpCas9-HF1 R832A and SpCas9HF1+K1014A) did not show an appreciable change in cleavage with the mismatched sgRNA. However, importantly, most of the SpCas9-HF1 derivatives had substantially lower activity with the 11/12 mismatched sgRNA than what was observed with SpCas9-HF1, eSpCas9(1.0), or eSpCas9(1.1), suggesting that certain combinations of these new variants have reduced mismatched-target activities and thus improved specificities (FIG. 14A). Of the 16 SpCas9-HF1 derivatives that reduced mismatChed-target activities with the 11/12 mismatched sgRNA to near background levels, 9 appeared to have only minimal effects on on-target activity (assessed using the perfectly matched sgRNA; FIG. 14A). Additional testing of a subset of these SpCas9-HF1 derivatives in the EGFP disruption assay using an sgRNA intentionally mismatched at positions 9 and 10 (FIG. 14B) also revealed that these variants possessed lower activities with this mismatched sgRNA than what was observed either with SpCas9-HF1 (FIG. 14b ), with eSpCas9(1.1) (FIG. 13A), or with the same substitutions added to wild-type SpCas9 nuclease (FIG. 13B). Importantly, five variants showed background level off-target activity in this assay with the 9/10 mismatched sgRNA.

Next, whether these alanine substitutions of the non-target strand could be combined with the SpCas9 variant that contains only the Q695A and Q9264 substitutions from our SpCas9-HF1 variant (here “double” variant) was tested. Because many of the HF1 derivatives tested above showed an observable (and undesirable) decrease in on-target activity, it was hypothesized that combining only the two most important substitutions from SpCas9-HF1 (Q695A and Q926A; see FIG. 1B) with one or more non-target strand contacting substitutions might rescue on-target activity but still maintain the gains in specificity observed when these substitutions were added to the SpCas9-H.F1 variant. Therefore, various SpCas9(Q695A/Q926A) derivatives bearing combinations of single, double, or triple alanine substitutions at potential non-target DNA strand interacting positions were tested in the human cell-based EGFP disruption assay using the same perfectly matched sgRNA targeted to EGFP described above (to test on-target activities) and the same sgRNA bearing mismatches at positions 11 and 12 (to assess activities at a mismatched target site, as would be found for off-target sites) that were used for FIGS. 13A-B. This experiment revealed most of the SpCas9(Q695A/Q926A) derivative variants tested showed comparable on-target activities to those observed with both wild-type SpCas9 and SpCas9-HF (FIG. 15) Importantly, many of the SpCas9-HF1 derivatives had substantially lower activity with the 11/12 mismatched. sgRNA compared with what was observed with SpCas9-HF1, eSpCas9(1.0), or eSpCas9(1.1) suggesting that certain combinations of these new variants have reduced mismatched-target activities and thus improved specificities (FIG. 15). Of the 13 SpCas9(Q695A/Q926A) derivatives that reduced mismatched-target activities with the 11/12 mismatched sgRNA to near background levels, only 1 appeared to have a substantial effect on on-target activity (assessed using the perfectly matched sgRNA; FIG. 15).

Overall, these data demonstrate that the addition of one, two, or three alanine substitutions to SpCas9-HF1 or SpCas9(Q695A/Q926A) at positions that might contact the non-target DNA strand can lead to new variants with improved abilities to discriminate against mismatched off-target sites (relative to to their parental clones or the recently described eSpCas9(1.0) or (1.1). Importantly, these same substitutions in the context of wild-type SpCas9 do not appear to provide any substantial specificity benefit.

To better define and compare the tolerances of SpCas9-HF1 and eSpCas9-1.1 to mismatches at the sgRNA-target DNA complementarily interface, their activities were examined using sgRNAs containing single mismatches at all possible positions in the spacer complementarity region. Both the SpCas9-HF1and eSPCas9-1.1 variants had similar activities on most singly mismatched sgRNAs when compared to wild-type SpCas9, with a few exceptions where SpCas9-HF1 outperformed eSpCas9-1.1 (FIG. 16).

Next we tested the single nucleotide mismatch tolerance of some variants containing combinations of amino acid substitutions from either the double mutant (Db=Q695A/Q926A), SpCas9-HF1 (N497A/R661A/Q695A/Q926A), eSpCas9-1.0 (1.0=K810A/K1003A/R1060A), or eSpCas9-1.1(1.1=K848A/K1003A/R1060A) with additional alanine substitutions in residues that contact the target strand DNA or that potentially contact the non-target strand DNA (FIGS. 17A-B). On-target activity was assessed using a perfectly matched sgRNA, while single nucleotide mismatch tolerance was assessed using sgRNAs bearing such mismatches at positions 4, 8, 12, or 16 in the spacer sequence (FIG. 17A). A number of these variants maintained on-target activity with substantial reductions in activities observed with the mismatched sgRNAs. Three of these variants (0695A/K848A/Q926A/K1003A/R1060A, N497A/R661A/Q695A/K855A/Q926A/R1060A, and N497A/R661A/Q695A/Q926A/H982A/R1060A) were further tested with the remaining single mismatch sgRNAs (containing mismatches at positions 1-3, 5-7, 9-11, 13-15, and 17-20). These variants demonstrated a more robust intolerance to single nucleotide substitutions in the sgRNA compared with eSpCas9-1.1, demonstrating the improved specificity profile of these new variants (FIG. 17B), Additional variant nucleases containing alternative combinations of amino acid substitutions were tested using sgRNAs containing mismatches at positions 5, 7, and 9 in the spacer (these particular mismatched sgRNAs were used because earlier variants appeared to tolerate mismatches at these positions) (FIG. 18) A number of these nucleases had improved specificities against the mismatched sites, with only marginal reductions in on-target activities (FIG. 18).

To further determine whether additional combinations of mutations could convey specificity improvements, a greatly expanded panel of nuclease variants with two additional matched sgRNAs was tested to examine on-target activity in our EGFP disruption activity (FIG. 19A). A number of these variants maintained robust on-target activities, suggesting that they may be useful for generating further improvements to specificity (FIG. 19B). A number of these variants were tested with sgRNAs containing single substitutions at positions 12, 14, 16, or 18 to determine whether specificity improvements were observed and were found to exhibit greater intolerance to single nucleotide mismatches at these positions (FIG. 19B).

Example 3

Taking an analogous strategy with Staphylococcus aureus Cas9 (SaCas9) as we had done with SpCas9, experiments were performed to improve the specificity of SaCas9 by introducing alanine substitutions in residues that are known to contact the target DNA strand (FIG. 20 and FIG. 21A), residues that may contact the non-target DNA (ongoing experiments), and residues that we have previously shown can influence PAM specificity (FIG. 21B). Residues that may contact the target strand DNA backbone include: Y211, Y212, W229, Y230, R245, T392, N419, L446, Y651, and R654; residues that may contact the non-target strand DNA include: Q848, N492, Q495, R497, N498, R499, Q500, K518, K523, K525, H557, R561, K572, R634, R654, G655, N658, S662, N668, R686, K692, R694,1-H700, K751; and residues that contact the PAM include: E782, D786, T787, Y789, T882, K886, N888, A889, L909, K929, N985, N986, R991, and R1015. In a preliminary experiment, single alanine substitutions (or some combinations thereof) in either target strand DNA contacting residues or PAM contacting residues (FIGS. 21A and B, respectively) had variable effects on on-target EGFP disruption activity (using a perfectly matched sgRNA) and were unable to eliminate off-target cleavage (when using an sgRNA mismatched at positions 11 and 12). Interestingly, SpCas9 mutations in the HF1 were unable to completely abolish off-target activity with a similarly mismatched target/sgRNA pair, suggesting that variants containing combinations of target strand/non-target strand substitutions may be necessary to improve specificity at such sites (as we observed with SpCas9).

To further assess the strategy of mutating potential target strand DNA contacts to improve SaCas9 specificity, the potential of single, double, triple, and quadruple combinations of mutations to tolerate mismatches at positions 19 and 20 in an sgRNA was examined (FIGS. 22A and B). These combinations revealed that alanine substitutions at Y230 and R245, when combined with other substitutions, can increase specificity as judged by the capability to better discriminate against mismatched sites.

Next the on-target gene disruption activities of two of these triple alanine substitution variants (Y211A/Y230A/R245A and Y212A/Y230A/R245A) were examined at 4 on-target sites in EGFP (matched sites #1-4 FIG. 23). These variants maintained robust on-target activities for matched sites 1 and 2 but showed approximately 60-70% loss of on-target activity with matched sites 3 and 4. Both of these triple alanine substitution variants dramatically improved specificity relative to wild-type SaCas9 as judged by using sgRNAs bearing double mismatches at various positions in the spacers of target sites 1-4 (FIG. 23).

SaCas9 variants bearing double and triple combinations (FIGS. 24A and B, respectively) of these alanine substitutions were tested on six endogenous sites for on target activities and improvements in specificity assessed using an sgRNA containing a single mismatch at position 21 (the most PAM distal position expected to be a challenging mismatch to discriminate against). In some cases, on-target activities with the matched sgRNA were maintained with the variants while ‘off-target’ activities with the sgRNA mismatched at position 21 were eliminated (FIGS. 24A and B). In other cases, marginal to complete loss of activity was observed with the matched sgRNA.

REFERENCES

-   1. Sander, J. D. & Joung, J. K. CRISPR-Cas systems for editing,     regulating and targeting genomes. Nat Biotechnol 32, 347-355 (2014). -   2. Hsu, P. D., Lander, E. S. & Zhang, F. Development and     applications of CRISPR-Cas9 for genome engineering. Cell 157,     1262-1278 (2014). -   3. Doudna, J. A. & Charpentier, E. Genome editing. The new frontier     of genome engineering with CRISPR-Cas9. Science 346, 1258096 (2014). -   4. Barrangou, R. & May, A. P. Unraveling the potential of     CRISPR-Cas9 for gene therapy. Expert Opin Biol Ther 15, 311-314     (2015). -   5. Jinek, M. et al. A programmable dual-RNA-guided DNA endonuclease     in adaptive bacterial immunity. Science 337, 816-821 (2012). -   6. Sternberg, S. H., Redding, S., Jinek, M., Greene, E. C. &     Doudna, J. A. DNA interrogation by the CRISPR RNA-guided     endonuclease Cas9. Nature 507, 62-67 (2014). -   7. Hsu, P. D. et al. DNA targeting specificity of RNA-guided Cas9     nucleases. Nat Biotechnol 31, 827-832 (2013). -   8. Tsai, S. Q. et al. GUIDE-seq enables genome-wide profiling of     off-target cleavage by CRISPR-Cas nucleases. Nat Biotechnol 33,     187-197 (2015). -   9. Hou, Z. et al. Efficient genome engineering in human pluripotent     stem cells using Cas9 from Neisseria meningitidis. Proc Natl Acad     Sci USA (2013). -   10. Fonfara., 1. et al. Phylogeny of Cas9 determines functional     exchangeability of dual-RNA and Cas9 among orthologous type II     CRISPR-Cas systems. Nucleic Acids Res 42, 2577-2590 (2014). -   11. Esvelt, K. M. et al. Orthogonal Cas9 proteins for RNA-guided     gene regulation and editing. Nat Methods 10, 1116-1121 (2013). -   12. Cong, L. et al. Multiplex genome engineering using CRISPR/Cas     systems. Science 339, 819-823 (2013) -   13. Horvath, P. et al. Diversity, activity, and evolution of CRISPR     loci in Streptococcus thermophilus, Bacteriol 190, 1401-1412 (2008). -   14. Anders, C., Niewoehner, O., Duerst, A. & Jinek, M. Structural     basis of PAM-dependent target DNA recognition by the Cas9     endonuclease. Nature 513, 569-573 (2014). -   15. Revon, D. et al. FLASH assembly of TALENs for high-throughput     genome editing. Nat Biotechnol 30, 460-465 (2012). -   16. Fu, Y. et al. High-frequency off-target mutagenesis induced by     CRISPR-Cas nucleases in human cells. Nat Biotechnol 31, 822-826     (2013). -   17. Chen, Z. & Zhao, H. A highly sensitive selection method for     directed evolution of homing endonucleases. Nucleic Acids Res 33, el     54 (2005). -   18. Doyon, J. B., Pattanayak, V., Meyer, C. B. & Liu, D. R. Directed     evolution and substrate specificity profile of homing endonuclease     I-Scer. J Am Chem Soc 128, 2477-2484 (2006). -   19. Jiang, W., Bikard, D., Cox, D., Zhang, F. & Marraffini, L. A.     RNA-guided editing of bacterial genomes using CRISPR-Cas systems.     Nat Biotechnol 31, 233-239 (2013). -   20. Mali, P. et al. RNA-guided human genome engineering via Cas9.     Science 339, 823-826 (2013). -   21 Hwang, W. Y. et al. Efficient genome editing in zebrafish using a     CRISPR-Cas system. Nat Biotechnol 31, 227-229 (2013), -   22. Chylinski, K., Le Rhun, A. & Charpentier, E. The tracrRNA and     Cas9 families of type II CRISPR-Cas immunity systems. RNA Biol 10,     726-737 (2013). -   23. Kleinstiver, B. P., Fernandes, A. D., (Moor, G. B. &     Edge'', D. R. A unified genetic, computational and experimental     framework identifies functionally relevant residues of the homing     endonuclease I-Bmol. Nucleic Acids Res 38, 2411-2427 (2010). -   24. Gagnon, J. A. et al. Efficient mutagenesis by Cas9     protein-mediated oligonucleotide insertion and large-scale     assessment of single-guide RNAs. PLoS One 9, e98186 (2014).

SEQUENCES

SEQ ID NO:271—JDS246: CMV-T7-humanSpCas9-NLS-3xFLAG

Human codon optimized S. pyogenes Cas9 in normal font, NLS double underlined, 3xFLAG tag in bold:

ATGGATAAAAAGTATTCTATTGGTTTAGACATCGG CACTAATTCCGTTGGATGGGCTGTCATAACCGAT GAATACAAAGTACCTTCAAAGAAATTTAAGGTGTT GGGGAACACAGACCGTCATTCGATTAAAAAGAAT CTTATCGGTGCCCTCCTATTCGATAGTGGCGAAAC GGCAGAGGCGACTCGCCTGAAACGAACCGCTCGG AGAAGGTATACACGTCGCAAGAACCGAATATGTTA CTTACAAGAAATTTTTAGCAATGAGATGGCCAAA GTTGACGATTCTTTCTTTCACCGTTTGGAAGAGTC CTTCCTTGTCGAAGAGGACAAGAAACATGAACGG CACCCCATCTTTGGAAACATAGTAGATGAGGTGGC ATATCATGAAAAGTACCCAACGATTTATCACCTC AGAAAAAAGCTAGTTGACTCAACTGATAAAGCGGA CCTGAGGTTAATCTACTTGGCTCTTGCCCATATG ATAAAGTTCCGTGGGCACTTTCTCATTGAGGGTGA TCTAAATCCGGACAACTCGGATGTCGACAAACTG TTCATCCAGTTAGTACAAACCTATAATCAGTTGTT TGAAGAGAACCCTATAAATGCAAGTGGCGTGGAT GCGAAGGCTATTCTTAGCGCCCGCCTCTCTAAATC CCGACGGCTAGAAAACCTGATCGCACAATTACCC GGAGAGAAGAAAAATGGGTTGTTCGGTAACCTTAT AGCGCTCTCACTAGGCCTGACACCAAATTTTAAG TCGAACTTCGACTTAGCTGAAGATGCCAAATTGCA GCTTAGTAAGGACACGTACGATGACGATCTCGAC AATCTACTGGCACAAATTGGAGATCAGTATGCGGA CTTATTTTTGGCTGCCAAAAACCTTAGCGATGCA ATCCTCCTATCTGACATACTGAGAGTTAATACTGA GATTACCAAGGCGCCGTTATCCGCTTCAATGATC AAAAGGTACGATGAACATCACCAAGACTTGACACT TCTCAAGGCCCTAGTCCGTCAGCAACTGCCTGAG AAATATAAGGAAATATTCTTTGATCAGTCGAAAAA CGGGTACGCAGGTTATATTGACGGCGGAGCGAGT CAAGAGGAATTCTACAAGTTTATCAAACCCATATT AGAGAAGATGGATGGGACGGAAGAGTTGCTTGTA AAACTCAATCGCGAAGATCTACTGCGAAAGCAGCG GACTTTCGACAACGGTAGCATTCCACATCAAATC CACTTAGGCGAATTGCATGCTATACTTAGAAGGCA GGAGGATTTTTATCCGTTCCTCAAAGACAATCGT GAAAAGATTGAGAAAATCCTAACCTTTCGCATACC TTACTATGTGGGACCCCTGGCCCGAGGGAACTCT CGGTTCGCATGGATGACAAGAAAGTCCGAAGAAAC GATTACTCCATGGAATTTTGAGGAAGTTGTCGAT AAAGGTGCGTCAGCTGAATCGTTCATCGAGAGGAT GACCAACTTTGACAAGAATTTACCGAACGAAAAA GTATTGCCTAAGCACAGTTTACTTTACGAGTATTT CACAGTGTACAATGAACTCACGAAAGTTAAGTAT GTCACTGAGGGCATGCGTAAACCCGCCTTTCTAAG CGGAGAACAGAAGAAAGCAATAGTAGATCTGTTA TTCAAGACCAACCGCAAAGTGACAGTTAAGCAATT GAAAGAGGACTACTTTAAGAAAATTGAATGCTTC GATTCTGTCGAGATCTCCGGGGTAGAAGATCGATT TAATGCGTCACTTGGTACGTATCATGACCTCCTA AAGATAATTAAAGATAAGGACTTCCTGGATAACGA AGAGAATGAAGATATCTTAGAAGATATAGTGTTG ACTCTTACCCTCTTTGAAGATCGGGAAATGATTGA GGAAAGACTAAAAACATACGCTCACCTGTTCGAC GATAAGGTTATGAAACAGTTAAAGAGGCGTCGCTA TACGGGCTGGGGACGATTGTCGCGGAAACTTATC AACGGGATAAGAGACAAGCAAAGTGGTAAAACTAT TCTCGATTTTCTAAAGAGCGACGGCTTCGCCAAT AGGAACTTTATGCAGCTGATCCATGATGACTCTTT AACCTTCAAAGAGGATATACAAAAGGCACAGGTT TCCGGACAAGGGGACTCATTGCACGAACATATTGC GAATCTTGCTGGTTCGCCAGCCATCAAAAAGGGC ATACTCGAGAC&GTCAAAGTAGTGGATGAGCTAGT TAAGGTCATGGGACGTCACAAACCGGAAAACATT GTAATCGAGATGGCACGCGAAAATCAAACGACTCA GAAGGGGCAAAAAAACAGTCGAGAGCGGATGAAG AGAATAGAAGAGGGTATTAAAGAACTGGGCAGCCA GATCTTAAAGGAGCATCCTGTGGAAAATACCCAA TTGCAGAACGAGAAACTTTACCTCTATTACCTACA AAATGGAAGGGACATGTATGTTGATCAGGAACTG GACATAAACCGTTTATCTGATTACGACGTCGATCA CATTGTACCCCAATCCTTTTTGAAGGACGATTCA ATCGAGAATAAAGTGCTTACACGCTCGGATAAGAA CCGAGGGAAAAGTGACAATGTTCGAAGCGAGGAA GTCGTAAAGAAAATGAAGAACTATTGGCGGCAGCT CCTAAATGCGAAACTGATAACGCAAAGAAAGTTC GATAACTTAACTAAAGCTGAGAGGGGTGGCTTGTC TGAACTTGACAAGGCCGGATTTATTAAACGTCAG CTCGTGGAAACCCGCCAAATCACAAAGCATGTTGC AAAGATACTAGATTCCCGAATGAATACGAAATAC GACGAGAACGATAAGCTGATTCGGGAAGTCAAAGT AATCACTTTAAAGTCAAAATTGGTGTCGGACTTC AGAAAGGATTTTCAATTCTATAAAGTTAGGGAGAT AAATAACTACCACCATGCGCACGACGCTTATCTT AATGCCGTCGTAGGGACCGCACTCATTAAGAAATA CCCGAAGCTAGAAAGTGAGTTTGTGTATGGTGAT TACAAAGTTTATGACGTCCGTAAGATGATCGCGAA AAGCGAACAGGAGATAGGCAAGGCTACAGCCAAA TACTTCTTTTATTCTAACATTATGAATTTCTTTAA GACGGAAATCACTCTGGCAAACGGAGAGATACGC AAACGACCTTTAATTGAAACCAATGGGGAGACAGG TGAAATCGTATGGGATAAGGGCCGGGACTTCGCG ACGGTGAGAAAAGTTTTGTCCATGCCCCAAGTCAA CATAGTAAAGAAAACTGAGGTGCAGACCGGAGGG TTTTCAAAGGAATCGATTCTTCCAAAAAGGAATAG TGATAAGCTCATCGCTCGTAAAAAGGACTGGGAC CCGAAAAAGTACGGTGGCTTCGATAGCCCTACAGT TGCCTATTCTGTCCTAGTAGTGGCAAAAGTTGAG AAGGGAAAATCCAAGAAACTGAAGTCAGTCAAAGA ATTATTGGGGATAACGATTATGGAGCGCTCGTCT TTTGAAAAGAACCCCATCGACTTCCTTGAGGCGAA AGGTTACAAGGAAGTAAAAAAGGATCTCATAATT AAACTACCAAAGTATAGTCTGTTTGAGTTAGAAAA TGGCCGAAAACGGATGTTGGCTAGCGCCGGAGAG CTTCAAAAGGGGAACGAACTCGCACTACCGTCTAA ATACGTGAATTTCCTGTATTTAGCGTCCCATTAC GAGAAGTTGAAAGGTTCACCTGAAGATAACGAACA GAAGCAACTTTTTGTTGAGCAGCACAAACATTAT CTCGACGAAATCATAGAGCAAATTTCGGAATTCAG TAAGAGAGTCATCCTAGCTGATGCCAATCTGGAC AAAGTATTAAGCGCATACAACAAGCAGAGGGATAA ACCCATACGTGAGCAGGCGGAAAATATTATCCAT TTGTTTACTCTTACCAACCTCGGCGCTCCAGCCGC ATTCAAGTATTTTGACACAACGATAGATCGCAAA CGATACACTTCTACCAAGGAGGTGCTAGACGCGAC ACTGATTCACCAATCCATCACGGGATTATATGAA ACTCGGATAGATTTGTCACAGCTTGGGGGTGACGG ATCCCCCAAGAAGAAGAGGAAAGTCTCGAGCGAC TACAAAGACCATGACGGTGATTATAAAGATCATGA CATCGATTACAAGGATGACGATGACAAGTGA

SEQ ID NO: 272—VP12: CMV-T7-humanSpCas9-HF1(N497A, R661A, Q695A, Q926A)-NLS-3xFLAG

Human codon optimized S. pyogenes Cas9 in normal font, modified codons in lower case, NLS double underlined, 3xFLAG tag in bold:

ATGGATAAAAAGTATTCTATTGGTTTAGACATCGG CACTAATTCCGTTGGATGGGCTGTCATAACCGAT GAATACAAAGTACCTTCAAAGAAATTTAAGGTGTT GGGGAACACAGACCGTCATTCGATTAAAAAGAAT CTTATCGGTGCCCTCCTATTCGATAGTGGCGAAAC GGCAGAGGCGACTCGCCTGAAACGAACCGCTCGG AGAAGGTATACACGTCGCAAGAACCGAATATGTTA CTTACAAGAAATTTTTAGCAATGAGATGGCCAAA GTTGACGATTCTTTCTTTCACCGTTTGGAAGAGTC CTTCCTTGTCGAAGAGGACAAGAAACATGAACGG CACCCCATCTTTGGAAACATAGTAGATGAGGTGGC ATATCATGAAAAGTACCCAACGATTTATCACCTC AGAAAAAAGCTAGTTGACTCAACTGATAAAGCGGA CCTGAGGTTAATCTACTTGGCTCTTGCCCATATG ATAAACTTCCGTGGGCACTTTCTCATTGAGGGTGA TCTAAATCCGGACAACTCGGATCTCGACAAACTG TTCATCCAGTTAGTACAAACCTATAATCAGTTGTT TGAAGAGAACCCTATAAATGCAAGTGGCGTGGAT GCGAAGGCTATTCTTAGCGCCCGCCTCTCTAAATC CCGACGGCTAGAAAACCTGATCGCACAATTACCC GGAGAGAAGAAAAATGGGTTGTTCGGTAACCTTAT AGCGCTCTCACTAGGCCTGACACCAAATTTTAAG TCGAACTTCGACTTAGCTGAAGATGCCAAATTGCA GCTTAGTAAGGACACGTACGATGACGATCTCGAC AATCTACTGGCACAAATTGGAGATCAGTATGCGGA CTTATTTTTGGCTGCCAAAAACCTTAGCGATGCA ATCCTCCTATCTGACATACTGAGAGTTAATACTGA GATTACCAAGGCGCCGTTATCCGCTTCAATGATC AAAAGGTACGATGAACATCACCAAGACTTGACACT TCTCAAGGCCCTAGTCCGTCAGCAACTGCCTGAG AAATATAAGGAAATATTCTTTGATCAGTCGAAAAA CGGGTACGCAGGTTATATTGACGGCGGAGCGAGT CAAGAGGAATTCTACAAGTTTATCAAACCCATATT AGAGAAGATGGATGGGACGGAAGAGTTGCTTGTA AAACTCAATCGCGAAGATCTACTGCGAAAGCAGCG GACTTTCGACAACGGTAGCATTCCACATCAAATC CACTTAGGCGAATTGCATGCTATACTTAGAAGGCA GGAGGATTTTTATCCGTTCCTCAAAGACAATCGT GAAAAGATTGAGAAAATCCTAACCTTTCGCATACC TTACTATGTGGGACCCCTGGCCCGAGGGAACTCT CGGTTCGCATGGATGACAAGAAAGTCCGAAGAAAC GATTACTCCCTGGAATTTTGAGGAAGTTGTCGAT AAAGGTGCGTCAGCTCAATCGTTCATCGAGAGGAT GACCgccTTTGACAAGAATTTACCGAACGAAAAA GTATTGCCTAAGCACAGTTTACTTTACGAGTATTT CACAGTGTACAATGAACTCACGAAAGTTAAGTAT GTCACTGAGGGCATGCGTAAACCCGCCTTTCTAAG CGGAGAACAGAAGAAAGCAATAGTAGATCTGTTA TTCAAGACCAACCGCAAAGTGACAGTTAAGCAATT GAAAGAGGACTACTTTAAGAAAATTGAATGCTTC GATTCTGTCGAGATCTCCGGGGTAGAAGATCGATT TAATGCGTCACTTGGTACGTATCATGACCTCCTA AAGATAATTAAAGATAAGGACTTCCTGGATAACGA AGAGAATGAAGATATCTTAGAAGATATAGTGTTG ACTCTTACCCTCTTTGAAGATCGGGAAATGATTGA GGAAAGACTAAAAACATACGCRCACCTGTTCGAC GATAAGGTTATGAAACAGTTAAAGAGGCGTCGCTA TACGGGCTGGGGAgccTTGTCGCGGAAACTTATC AACGGGATAAGAGACAAGCAAAGTGGTAAAACTAT TCTCGATTTTCTAAAGAGCGACGGCTTCGCCAAT AGGAACTTTATGgccCTGATCCATGATGACTCTTT AACCTTCAAAGAGGATATACAAAAGGCACAGGTT TCCGGACAAGGGGACTCATTGCACGAACATATTGC GAATCTTGCTGGTTCGCCAGCCATCAAAAAGGGC ATACTCCAGACAGTCAAAGTAGTGGATGAGCTAGT TAAGGTCATGGGACGTCACAAACCGGAAAACATT GTAATCGAGATGGCACGCGAAAATCAAACGACTCA GAAGGGGCAAAAAAACAGTCGAGAGCGGATGAAG AGAATAGAAGAGGGTATTAAAGAACTGGGCAGCCA GATCTTAAAGGAGCATCCTGTGGAAAATACCCAA TTGCAGAACGAGAAACTTTACCTCTATTACCTACA AAATGGAAGGGACATGTATGTTGATCAGGAACTG GACATAAACCGTTTATCTGATTACGACGTCGATCA CATTGTACCCCAATCCTTTTTGAAGGACGATTCA ATCGACAATAAAGTGCTTACACGCTCGGATAAGAA CCGAGGGAAAAGTGACAATGTTCCAAGCGAGGAA GTCGTAAAGAAAATGAAGAACTATTGGCGGCAGCT CCTAAATGCGAAACTGATAACGCAAAGAAAGTTC GATAACTTAACTAAAGCTGAGAGGGGTGGCTTGTC TGAACTTGACAAGGCCGGATTTATTAAACGTCAG CTCGTGGAAACCCGCGCCATCACAAAGCATGTTGC GCAGATACTAGATTCCCGAATGAATACGAAATAC GACGAGAACGATAAGCTGATTCGGGAAGTCAAAGT AATCACTTTAAAGTCAAAATTGGTGTCGGACTTC AGAAAGGATTTTCAATTCTATAAAGTTAGGGAGAT AAATAACTACCACCATGCGCACGACGCTTATCTT AATGCCGTCGTAGGGACCGCACTCATTAAGAAATA CCCGAAGCTAGAAAGTGAGTTTGTGTATGGTGAT TACAAAGTTTATGACGTCCGTAAGATGATCGCGAA AAGCGAACAGGAGATAGGCAAGGCTACAGCCAAA TACTTCTTTTATTCTAACATTATGAATTTCTTTAA GACGGAAATCACTCTGGCAAACGGAGAGATACGC AAACGACCTTTAATTGAAACCAATGGGGAGACAGG TGAAARCGTATGGGATAAGGGCCGGGACTTCGCG ACGGTGAGAAAAGTTTTGTCCATGCCCCAAGTCAA CATAGTAAAGAAAACTGAGGTGCAGACCGGAGGG TTTTCAAAGGAATCGATTCTTCCAAAAAGGAATAG TGATAAGCTCATCGCTCGTAAAAAGGACTGGGAC CCGAAAAAGTACGGTGGCTTCGATAGCCCTACAGT TGCCTATTCTGTCCTAGTAGTGGCAAAAGTTGAG AAGGGAAAATCCAAGAAACTGAAGTCAGTCAAAGA ATTATTGGGGATAACGATTATGGAGCGCTCGTCT TTTGAAAAGAACCCCATCGACTTCCTTGAGGCGAA AGGTTACAAGGAAGTAAAAAAGGATCTCATAATT AAACTACCAAAGTATAGTCTGTTTGAGTTAGAAAA TGGCCGAAAACGGATGTTGGCTAGCGCCGGAGAG CTTCAAAAGGGGAACGAACTCGCACTACCGTCTAA ATACGTGAATTTCCTGTATTTAGCGTCCCATTAC GAGAAGTTGAAAGGTTCACCTGAAGATAACGAACA GAAGCAACTTTTTGTTGAGCAGCACAAACATTAT CTCGACGAAATCATAGAGCAAATTTCGGAATTCAG TAAGAGAGTCATCCTAGCTGATGCCAATCTGGAC AAAGTATTAAGCGCATACAACAAGCACAGGGATAA ACCCATACGTGAGCAGGCGGAAAATATTATCCAT TTGTTTACTCTTACCAACCTCGGCGCTCCAGCCGC ATTCAAGTATTTTGACACAACGATAGATCGCAAA CGATACACTTCTACCAAGGAGGTGCTAGACGCGAC ACTGATTCACCAATCCATCACGGGATTATATGAA ACTCGGATAGATTTGTCACAGCTTGGGGGTGACGG ATCCCCCAAGAAGAAGAGGAAAGTCTCGAGCGAC TACAAAGACCATGACGGTGATTATAAAGATCATGA CATCGATTACAAGGATGACGATGACAAGTGA

SEQ ID NO:273—MSP2135: CMV-T7-humanSpCas9 HF7(N497A, R661A, Q695A, Q926A, D1135E)-NLS-3xFLAG

Human codon optimized S. pyogenes Cas9 in normal font, modified codons in lower case, NLS double underlined, 3xFLAG tag in bold:

ATGGATAAAAAGTATTCTATTGGTTTAGACATCGG CACTAATTCCGTTGGATGGGCTGTCATAACCGAT GAATACAAAGTACCTTCAAAGAAATTTAAGGTGTT GGGGAAGACAGACCGTCATTCGATTAAAAAGAAT CTTATCGGTGCCCTCCTATTCGATAGTGGCGAAAC GGCAGAGGCGACTCGCCTGAAACGAACCGCTCGG AGAAGGTATACACGTCGCAAGAACCGAATATGTTA CTTACAAGAAATTTTTAGCAATGAGATGGCCAAA GTTGACGATTCTTTCTTTCACCGTTTGGAAGAGTC CTTCCTTGTCGAAGAGGACAAGAAACATGAACGG CACCCCATCTTTGGAAACATAGTAGATGAGGTGGC ATATCATGAAAAGTACCCAACGATTTATCACCTC AGAAAAAAGCTAGTTGACTCAACTGATAAAGCGGA CCTGAGGTTAATCTACTTGGCTCTTGCCCATATG ATAAAGTTCCGTGGGCACTTTCTCATTGAGGGTGA TCTAAATCCGGACAACTCGGATGTCGACAAACTG TTCATCCAGTTAGTACAAACCTATAATCAGTTGTT TGAAGAGAACCCTATAAATGCAAGTGGCGTGGAT GCGAAGGCTATTCTTAGCGCCCGCCTCTCTAAATC CCGACGGCTAGAAAACCTGATCGCACAATTACCC GGAGAGAAGAAAAATGGGTTGTTCGGTAACCTTAT AGCGCTCTCACTAGGCCTGACACCAAATTTTAAG TCGAACTTCGACTTAGCTGAAGATGCCAAATTGCA GCTTAGTAAGGACACGTACGATGACGATCTCGAC AATCTACTGGCACAAATTGGAGATCAGTATGCGGA CTTATTTTTGGCTGCCAAAAACCTTAGCGATGCA ATCCTCCTATCTGACATACTGAGAGTTAATACTGA GATTACCAAGGCGCCGTTATCCGCTTCAATGATC AAAAGGTACGATGAACATCACCAAGACTTGACACT TCTCAAGGCCCTAGTCCGTCAGCAACTGCCTGAG AAATATAAGGAAATATTCTTTGATCAGTCGAAAAA CGGGTACGCAGGTTATATTGACGGCGGAGCGAGT CAAGAGGAATTCTACAAGTTTATCAAACCCATATT AGAGAAGATGGATGGGACGGAAGAGTTGCTTGTA AAACTCAATCGCGAAGATCTACTGCGAAAGCAGCG GACTTTCGACAACGGTAGCATTCCACATCAAATC CACTTAGGCGAATTGCATGCTATACTTAGAAGGCA GGAGGATTTTTATCCGTTCCTCAAAGACAATCGT GAAAAGATTGAGAAAATCCTAACCTTTCGCATACC TTACTATGTGGGACCCCTGGCCCGAGGGAACTCT CGGTTCGCATGGATGACAAGAAAGTCCGAAGAAAC GATTACTCCCTGGAATTTTGAGGAAGTTGTCGAT AAAGGTGCGTCAGCTCAATCGTTCATCGAGAGGAT GACCgccTTTGACAAGAATTTACCGAACGAAAAA GTATTGCCTAAGCACAGTTTACTTTACGAGTATTT CACAGTGTACAATGAACTCACGAAAGTTAAGTAT GTCACTGAGGGCATGCGTAAACCCGCCTTTCTAAG CGGAGAACAGAAGAAAGCAATAGTAGATCTGTTA TTCAAGACCAACCGCAAAGTGACAGTTAAGCAATT GAAAGAGGACTACTTTAAGAAAATTGAATGCTTC GATTCTGTCGAGATCTCCGGGGTAGAAGATCGATT TAATGCGTCACTTGGTACGTATCATGACCTCCTA AAGATAATTAAAGATAAGGACTTCCTGGATAACGA AGAGAATGAAGATATCTTAGAAGATATAGTGTTG ACTCTTACCCTCTTTGAAGATCGGGAAATGATTGA GGAAAGACTAAAAACATACGCTCACCTGTTCGAC GATAAGGTTATGAAACAGTTAAAGAGGCGTCGCTA TACGGGCTGGGGAgccTTGTCGCGGAAACTTATC AACGGGATAAGAGACAAGCAAAGTGGTAAAACTAT TCTCGATTTTCTAAAGAGCGACGGCTTCGCCAAT AGGAACTTTATGgccCTGATCCATGATGACTCTTT AACCTTCAAAGAGGATATACAAAAGGCACAGGTT TCCGGACAAGGGGACTCATTGCACGAACATATTGC GAATCTTGCTGGTTCGCCAGCCATCAAAAAGGGC ATACTCCAGACAGTCAAAGTAGTGGATGAGCTAGT TAAGGTCATGGGACGTCACAAACCGGAAAACATT GTAATCGAGATGGCACGCGAAAATCAAACGACTCA GAAGGGGCAAAAAAACAGTCGAGAGCGGATGAAG AGAATAGAAGAGGGTATTAAAGAACTGGGCAGCCA GATCTTAAAGGAGCATCCTGTGGAAAATACCCAA TTGCAGAACGAGAAACTTTACCTCTATTACCTACA AAATGGAAGGGACATGTATGTTGATCAGGAACTG GACATAAACCGTTTATCTGATTACGACGTCGATCA CATTGTACCCCAATCCTTTTTGAAGGACGATTCA ATCGACAATAAAGTGCTTACACGCTCGGATAAGAA CCGAGGGAAAAGTGACAATGTTCCAAGCGAGGAA GTCGTAAAGAAAATGAAGAACTATTGGCGGCAGCT CCTAAATGCGAAACTGATAACGCAAAGAAAGTTC GATAACTTAACTAAAGCTGAGAGGGGTGGCTTGTC TGAACTTGACAAGGCCGGATTTATTAAACGTCAG CTCGTGGAAACCCGCgccATCACAAAGCATGTTGC GCAGATACTAGATTCCCGAATGAATACGAAATAC GACGAGAACGATAAGCTGATTCGGGAAGTCAAAGT AATCACTTTAAAGTCAAAATTGGTGTCGGACTTC AGAAAGGATTTTCAATTCTATAAAGTTAGGGAGAT AAATAACTACCACCATGCGCACGACGCTTATCTT AATGCCGTCGTAGGGACCGCACTCATTAAGAAATA CCCGAAGCTAGAAAGTGAGTTTGTGTATGGTGAT TACAAAGTTTATGACGTCCGTAAGATGATCGCGAA AAGCGAACAGGAGATAGGCAAGGCTACAGCCAAA TACTTCTTTTATTCTAACATTATGAATTTCTTTAA GACGGAAATCACTCTGGCAAACGGAGAGATACGC AAACGACCTTTAATTGAAACCAATGGGGAGACAGG TGAAATCGTATGGGATAAGGGCCGGGACTTCGCG ACGGTGAGAAAAGTTTTGTCCATGCCCCAAGTCAA CATAGTAAAGAAAACTGAGGTGCAGACCGGAGGG TTTTCAAAGGAATCGATTCTTCCAAAAAGGAATAG TGATAAGCTCATCGCTCGTAAAAAGGACTGGGAC CCGAAAAAGTACGGTGGCTTCgagAGCCCTACAGT TGCCTATTCTGTCCTAGTAGTGGCAAAAGTTGAG AAGGGAAAATCCAAGAAACTGAAGTCAGTCAAAGA ATTATTGGGGATAACGATTATGGAGCGCTCGTCT TTTGAAAAGAACCCCATCGACTTCCTTGAGGCGAA AGGTTACTAGGAAGTAAAAAAGGATCTCATAATT AAACTACCAAAGTATAGTCTGTTTGAGTTAGAAAA TGGCCGAAAACGGATGTTGGCTAGCGCCGGAGAG CTTCAAAAGGGGAACGAACTCGCACTACCGTCTAA ATACGTGAATTTCCTGTATTTAGCGTCCCATTAC GAGAAGTTGAAAGGTTCACCTGAAGATAACGAACA GAAGCAACTTTTTGTTGAGCAGCACAAACATTAT CTCGACGAAATCATAGAGCAAATTTCGGAATTCAG TAAGAGAGTCATCCTAGCTGATGCCAATCTGGAC AAAGTATTAAGCGCATACAACAAGCACAGGGATAA ACCCATACGTGAGCAGGCGGAAAATATTATCCAT TTGTTTACTCTTACCAACCTCGGCGCTCCAGCCGC ATTCAAGTATTTTGACACAACGATAGATCGCAAA CGATACACTTCTACCAAGGAGGTGCTAGACGCGAC ACTGATTCACCAATCCATCACGGGATTATATGAA ACTCGGATAGATTTGTCACAGCTTGGGGGTGACGG ATCCCCCAAGAAGAAGAGGAAAGTCTCGAGCGAC TACAAAGACCATGACGGTGATTATAAAGATCATGA CATCGATTACAAGGATGACGATGACAAGTGA

SEQ ID NO:274—MSP2133: CMV-T7-humanSpCas9-HF4(Y450A, N497A, R661A, Q695A, Q926A)-NLS-3xFLAG

Human codon optimized S. pyogenes Car9 in normal font, modified codons in lower case, NLS double underlined, 3xFLAG tag in bold:

ATGGATAAAAAGTATTCTATTGGTTTAGACATCGG CACTAATTCCGTTGGATGGGCTGTCATAACCGAT GAATACAAAGTACCTTCAAAGAAATTTAAGGTGTT GGGGAACACAGACCGTCATTCGATTAAAAAGAAT CTTATCGGTGCCCTCCTATTCGATAGTGGCGAAAC GGCAGAGGCGACTCGCCTGAAACGAACCGCTCGG AGAAGGTATACACGTCGCAAGAACCGAATATGTTA CTTACAAGAAATTTTTAGCAATGAGATGGCCAAA GTTGACGATTCTTTCTTTCACCGTTTGGAAGAGTC CTTCCTTGTCGAAGAGGACAAGAAACATGAACGG CACCCCATCTTTGGAAACATAGTAGATGAGGTGGC ATATCATGAAAAGTACCCAACGATTTATCACCTC AGAAAAAAGCTAGTTGACTCAACTGATAAAGCGGA CCTGAGGTTAATCTACTTGGCTCTTGCCCATATG ATAAAGTTCCGTGGGCACTTTCTCATTGAGGGTGA TCTAAATCCGGACAACTCGGATGTCGACAAACTG TTCATCCAGTTAGTACAAACCTATAATCAGTTGTT TGAAGAGAACCCTATAAATGCAAGTGGCGTGGAT GCGAAGGCTATTCTTAGCGCCCGCCTCTCTAAATC CCGACGGCTAGAAAACCTGATCGCACAATTACCC GGAGAGAAGAAAAATGGGTTGTTCGGTAACCTTAT AGCGCTCTCACTAGGCCTGACACCAAATTTTAAG TCGAACTTCGACTTAGCTGAAGATGCCAAATTGCA GCTTAGTAAGGACACGTACGATGACGATCTCGAC AATCTACTGGCACAAATTGGAGATCAGTATGCGGA CTTATTTTTGGCTGCCAAAAACCTTAGCGATGCA ATCCTTCCTATCTGACATACTGAGAGTTAATACTC AGATTACCAAGGCGCCGTTATCCGCTTCATGATC AAAAGGTACGATGAACATCACCAAGACTTGACACT TCTCAAGGCCCTAGTCCGTCAGCAACTGCCTGAG AAATATAAGGAAATATTCTTTGATCAGTCGAAAAA CGGGTACGCAGGTTATATTGACGGCGGAGCGAGT CAAGAGGAATTCTACAAGTTTATCAAACCCATATT AGAGAAGATGGATGGGACGGAAGAGTTGCTTGTA AAACTCAATCGCGAAGATCTACTGCGAAAGCAGCG GACTTTCGACAACGGTAGCATTCCACATCAAATC CACTTAGGCGAATTGCATGCTATACTTAGAAGGCA GGAGGATTTTTATCCGTTCCTCAAAGACAATCGT GAAAAGATTGAGAAAATCCTAACCTTTCGCATACC TgccTATGTGGGACCCCTGGCCCGAGGGAACTCT CGGTTCGCATGGATGACAAGAAAGTCCGAAGAAAC GATTACTCCCTGGAATTTTGAGGAAGTTGTCGAT AAAGGTGCGTCAGCTCAATCGTTCATCGAGAGGAT GACCgccTTTGACAAGAATTTACCGAACGAAAAA GTATTGCCTAAGCACAGTTTACTTTACGAGTATTT CACAGTGTACAATGAACTCACGAAAGTTAAGTAT GTCACTGAGGGCATGCGTAAACCCGCCTTTCTAAG CGGAGAACAGAAGAAAGCAATAGTAGATCTGTTA TTCAAGACCAACCGCAAAGTGACAGTTAAGCAATT GAAAGAGCACTACTTTAAGAAAATTGAATGCTTC GATTCTGTCGAGATCTCCGGGGTAGAAGATCGATT TAATGCGTCACTTGGTACGTATCATGACCTCCTA AAGATAATTAAAGATAAGGACTTCCTGGATAACGA AGAGAATGAAGATATCTTAGAAGATATAGTGTTG ACTCTTACCCTCTTTGAAGATCGGGAAATGATTGA GGAAAGACTAAAAACATACGCTCACCTGTTCGAC GATAAGGTTATGAAACAGTTAAAGAGGCGTCGCTA TACGGGCTGGGGAgccTTGTCGCGGAAACTTATC AACGGGATAAGAGACAAGCAAAGTGGTAAAACTAT TCTCGATTTTCTAAAGAGCGACGGCTTCGCCAAT AGGAACTTTATGgccCTGATCCATGATGACTCCTT AACCTTCAAAGAGGATATACAAAAGGCACAGGTT TCCGGACAAGGGGACTCATTGCACGAACATATTGC GAATCTTGCTGGTTCGCCAGCCATCAAAAAGGGC ATACTCCAGACAGTCAAAGTAGTGGATGAGCTAGT TAAGGTCATGGGACGTCACAAACCGGAAAACATT GTAATCGAGATGGCACGCGAAAATCAAACGACTCA GAAGGGGCAAAAAAACAGTCGAGAGCGGATGAAG AGAATAGAAGAGGGTATTAAAGAACTGGGCAGCCA GATCTTAAAGGAGCATCCTGTGGAAAATACCCAA TTGCAGAACGAGAAACTTTACCTCTATTACCTACA AAATGGAAGGGACATGTATGTTGATCAGGAACTG GACATAAACCGTTTATCTGATTACGACGTCGATCA CATTGTACCCCAATCCTTTTTGAAGGACGATTCA ATCGACAATAAAGTGCTTACACGCTCGGATAAGAA CCGAGGGAAAAGTGACAATGTTCCAAGCGAGGAA GTCGTAAAGAAAATGAAGAACTATTGGCGGCAGCT CCTAAATGCGAAACTGATAACGCAAAGAAAGTTC GATAACTTAACTAAAGCTGAGAGGGGTGGCTTGTC TGAACTTGACAAGGCCGGATTTATTAAACGTCAG CTCGTGGAAACCCGCGCCATCACAAAGCATGTTCC GCAGATACTAGATTCCCGAATGAATACGAAATAC GACGAGAACGATAAGCTGATTCGGGAAGTCAAAGT AATCACTTTAAAGTCAAAATTGGTGTCGGACTTC AGAAAGGATTTTCAATTCTATAAAGTTAGGGAGAT AAATAACTACCACCATGCGCACGACGCTTATCTT AATGCCGTCGTAGGGACCGGACTCATTAAGAAATA CCCGAAGCTAGAAAGTGAGTTTGTGTATGGTGAT TACAAAGTTTATGACGTCCGTAAGATGATCGCGAA AAGCGAACAGGAGATAGGCAAGGCTACAGCCAAA TACTTCTTTTATTCTAACATTATGAATTTCTTTAA GACGGAAATCACTCTGGCAAACGGAGAGATACGC AAACGACCTTTAATTGAAACCAATGGGGAGACAGG TGAAATCGTATGGGATAAGGGCCGGGACTTCGCG ACGGTGAGAAAAGTTTTGTCCATGCCCCAAGTCAA CATAGTAAAGAAAACTGAGGTGCAGACCGGAGGG TTTTCAAAGGAATCGATTCTTCCAAAAAGGAATAG TGATAAGCTGATCGCTCGTAAAAAGGACTGGGAC CCGAAAAAGTACGGTGGCTTCGATAGCCCTACAGT TGCCTATTCTGTCCTAGTAGTGGCAAAAGTTGAG AAGGGAAAATCCAAGAAACTGAAGTCAGTCAAAGA ATTATTGGGGATAACGATTATGGAGCGCTCGTCT TTTGAAAAGAACCCCATCGACTTCCTTGAGGCGAA AGGTTACAAGGAAGTAAAAAAGGATCTCATAATT AAACTACCAAAGTATAGTCTGTTTGAGTTAGAAAA TGGCCGAAAACGGATGTTGGCTAGCGCCGGAGAG CTTCAAAAGGGGAACGAACTCGCACTACCGTCTAA ATACGTGAATTTCCTGTATTTAGCGTCCCATTAC GAGAAGTTGAAAGGTTCACCTGAAGATAACGAACA GAAGCAACTTTTTGTTGAGCAGCACAAACATTAT CTCGACGAAATCATAGAGCAAATTTCGGAATTCAG TAAGAGAGTCATCCTAGCTGATGCCAATCTGGAC AAAGTATTAAGCGCATACAACAAGCACAGGGATAA ACCCATACGTGAGCAGGCGGAAAATATTATCCAT TTGTTTACTCTTACCAACCTCGGCGCTCCAGCCGC ATTCAAGTATTTTGACACAACGATAGATCGCAAA CGATACACTTCTACCAAGGAGGTGCTAGACGCGAC ACTGATTCACCAATCCATCACGGGATTATATGAA ACTCGGATAGATTTGTCACAGCTTGGGGGTGACGG ATCCCCCAAGAAGAAGAGGAAAGTCTCGAGCGAC TACAAAGACCATGACGGTGATTATAAAGATCATGA CATCGATTACAAGGATGACGATGACAAGTGA

SEQ ID NO:275—MSP469: CMV-T7-humanSpCas9-VQR(D1135V, R1335Q, T1337R)-NLS-3xFLAG

Human codon optimized S. pyogenes Cas9 in normal font, modified codons in lower case, NLS double underlined, 3xFLAG tag in bold:

ATGGATAAAAAGTATTCTATTGGTTTAGACATCGG CACTAATTCCGTTGGATGGGCTGTCATAACCGAT GAATACAAAGTACCTTCAAAGAAATTTAAGGTGTT GGGGAACACAGACCGTCATTCGATTAAAAAGAAT CTTATCGGTGCCCTCCTATTCGATAGTGGCGAAAC GGCAGAGGCGACTCGCCTGAAACGAACCGCTCGG AGAAGGTATACACGTCGCAAGAACCGAATATGTTA CTTACAAGAAATTTTTAGCAATGAGATGGCCAAA GTTGACGATTCTTTCTTTCACCGTTTGGAAGAGTC CTTCCTTGTCGAAGAGGACAAGAAACATGAACGG CACCCCATCTTTGGAAACATAGTAGATGAGGTGGC ATATCATGAAAAGTACCCAACGATTTATCACCTC AGAAAAAAGCTAGTTGACTCAACTGATAAAGCGGA CCTGAGGTTAATCTACTTGGCTCTTGCCCATATG ATAAAGTTCCGTGGGCACTTTCTCATTGAGGGTGA TCTAAATCCGGACAACTCGGATGTCGACAAACTG TTCATCCAGTTAGTACAAACCTATAATCAGTTGTT TGAAGAGAACCCTATAAATGCAAGTGGCGTGGAT GCGAAGGCTATTCTTAGCGCCCGCCTCTCTAAATC CCGACGGCTAGAAAACCTGATCGCACAATTACCC GGAGAGAAGAAAAATGGGTTGTTCGGTAACCTTAT AGCGCTCTCACTAGGCCTGACACCAAATTTTAAG TCGAACTTCGACTTAGCTGAAGATGCCAAATTGCA GCTTAGTAAGGACACGTACGATGACGATCTCGAC AATCTACTGGCACAAATTGGAGATCAGTATGCGGA CTTATTTTTGGCTGCCAAAAACCTTAGCGATGCA ATCCTCCTATCTGACATACTGAGAGTTAATACTGA GATTACCAAGGCGCCGTTATCCGCTTCAATGATC AAAAGGTACGATGAACATCACCAAGACTTGACACT TCTCAAGGCCCTAGTCCGTCAGCAACTGCCTGAG AAATATAAGGAAATATTCTTTGATCAGTCGAAAAA CGGGTACGCAGGTTATATTGACGGCGGAGCGAGT CAAGAGGAATTCTACAAGTTTATCAAACCCATATT AGAGAAGATGGATGGGACGGAAGAGTTGCTTGTA AAACTCAATCGCGAAGATCTACTGCGAAAGCAGCG GACTTTCGACAACGGTAGCATTCCACATCAAATC CACTTAGGCGAATTGCATGCTATACTTAGAAGGCA GGAGGATTTTTATCCGTTCCTCAAAGACAATCGT GAAAAGATTGAGAAAATCCTAACCTTTCGCATACC TTACTATGTGGGACCCCTGGCCCGAGGGAACTCT CGGTTCGCATGGATGACAAGAAAGTCCGAAGAAAC GATTACTCCATGGAATTTTGAGGAAGTTGTCGAT AAAGGTGCGTCAGCTCAATCGTTCATCGAGAGGAT GACCAACTTTGACAAGAATTTACCGAACGAAAAA GTATTGCCTAAGCACAGTTTACTTTACGAGTATTT CACAGTGTACAATGAACTCACGAAAGTTAAGTAT GTCACTGAGGGCATGCGTAAACCCGCCTTTCTAAG CGGAGAACAGAAGAAAGCAATAGTAGATCTGTTA TTCAAGACCAACCGCAAAGTGACAGTTAAGCAATT GAAAGAGGACTACTTTAAGAAAATTGAATGCTTC GATTCTGTCGAGATCTCCGGGGTAGAAGATCGATT TAATGCGTCACTTGGTACGTATCATGACCTCCTA AAGATAATTAAAGATAAGGACTTCCTGGATAACGA AGAGAATGAAGATATCTTAGAAGATATAGTGTTG ACTCTTACCCTCTTTGAAGATCGGGAAATGATTGA GGAAAGACTAAAAACATACGCTCACCTGTTCGAC GATAAGGTTATGAAACAGTTAAAGAGGCGTCGCTA TACGGGCTGGGGACGATTGTCGCGGAAACTTATC AACGGGATAAGAGACAAGCAAAGTGGTAAAACTAT TCTCGATTTTCTAAAGAGCGACGGCTTCGCCAAT AGGAACTTTATGCAGCTGATCCATGATGACTCTTT AACCTTCAAAGAGGATATACAAAAGGCACAGGTT TCCGGACAAGGGGACTCATTGCACGAACATATTGC GAATCTTGCTGGTTCGCCAGCCATCAAAAAGGGC ATACTCCAGACAGTCAAAGTAGTGGATGAGCTAGT TAAGGTCATGGGACGTCACAAACCGGAAAACATT GTAATCGAGATGGCACGCGAAAATCAAACGACTCA GAAGGGGCAAAAAAACAGTCGAGAGCGGATGAAG AGAATAGAAGAGGGTATTAAAGAACTGGGCAGCCA GATCTTAAAGGAGCATCCTGTGGAAAATACCCAA TTGCAGAACGAGAAACTTTACCTCTATTACCTACA AAATGGAAGGGACATGTATGTTGATCAGGAACTG GACATAAACCGTTTATCTGATTACGACGTCGATCA CATTGTACCCCAATCCTTTTTGAAGGACGATTCA ATCGACAATAAAGTGCTTACACGCTCGGATAAGAA CCGAGGGAAAAGTGACAATGTTCCAAGCGAGGAA GTCGTAAAGAAAATGAAGAACTATTGGCGGCAGCT CCTAAATGCGAAACTGATAACGCAAAGAAAGTTC GATAACTTAACTAAAGCTGAGAGGGGTGGCTTGTC TGAACTTGACAAGGCCGGATTTATTAAACGTCAG CTCGTGGAAACCCGCCAAATCACAAAGCATGTTGC ACAGATACTAGATTCCCGAATGAATACGAAATAC GACGAGAACGATAAGCTCATTCGGGAAGTCAAAGT AATCACTTTAAAGTCAAAATTGGTGTCGGACTTC AGAAAGGATTTTCAATTCTATAAAGTTAGGGAGAT AAATAACTACCACCATGCGCACGACGCTTATCTT AATGCCGTCGTAGGGACCGCACTCATTAAGAAATA CCCGAAGCTAGAAAGTGAGTTTGTGTATGGTGAT TACAAAGTTTATGACGTCCGTAAGATGATCGCGAA AAGCGAACAGGAGATAGGCAAGGCTACAGCCAAA TACTTCTTTTATTCTAACATTATGAATTTCTTTAA GACGGAAATCACTCTGGCAAACGGAGAGATACGC AAACGACCTTTAATTGAAACCAATGGGGAGACAGG TGAAATCGTATGGGATAAGGGCCGGGACTTCGCG ACGGTGAGAAAAGTTTTGTCCATGCCCCAAGTCAA CATAGTAAAGAAAACTGAGGTGCAGACCGGAGGG TTTTCAAAGGAATCGATTCTTCCAAAAAGGAATAG TGATAAGCTCATCGCTCGTAAAAAGGACTGGGAC CCGAAAAAGTACGGTGGCTTCgtgAGCCCTACAGT TGCCTATTCTGTCCTAGTAGTGGCAAAAGTTGAG AAGGGAAAATCCAAGAAACTGAAGTCAGTCAAAGA ATTATTGGGGATAACGATTATGGAGCGCTCGTCT TTTGAAAAGAACCCCATCGACTTCCTTGAGGCGAA AGGTTACAAGGAAGTAAAAAAGGATCTCATAATT AAACTACCAAAGTATAGTCTGTTTGAGTTAGAAAA TGGCCGAAAACGGATGTTGGCTAGCGCCGGAGAG CTTCAAAAGGGGAACGAACTCGCACTACCGTCTAA ATACGTGAATTTCCTGTATTTAGCGTCCCATTAC GAGAAGTTGAAAGGTTCACCTGAAGATAACGAACA GAAGCAACTTTTTGTTGAGCAGCACAAACATTAT CTCGACGAAATCATAGAGCAAATTTCGGAATTCAG TAAGAGAGTCATCCTAGCTGATGCCAATCTGGAC AAAGTATTAAGCGCATACAACAAGCACAGGGATAA ACCCATACGTGAGCAGGCGGAAAATATTATCCAT cagTACagaTCTACCAAGGAGGTGCTAGACGCCAC ACTGATTCACCAATCCATCACGGGATTATATGAA ACTCGGATAGATTTGTCACAGCTTGGGGGTGACGG ATCCCCCAAGAAGAAGAGGAAAGTCTCGAGCGAC TACAAAGACCATGACGGTGATTATAAAGATCATGA CATCGATTACAAGGATGACGATGACAAGTGA

SEQ ID NO:276—MSP2440: CMV-T7-humanSpCas9-VQR-HF1(N497A, R661A, Q695A, Q926A, D1135V, R1335Q, T1337R)-NLS-3xFLAG

Human codon optimized S. pyogenes Cas9 in normal font, modified codons in lower case, NLS double underlined, 3xFLAG tag in bold:

ATGGATAAAAAGTATTCTATTGGTTTAGACATCGG CACTAATTCCGTTGGATGGGCTGTCATAACCGAT GAATACAAAGTACCTTCAAAGAAATTTAAGGTGTT GGGGAACACAGACCGTCATTCGATTAAAAAGAAT CTTATCGGTGCCCTCCTATTCGATAGTGGCGAAAC GGCAGAGGCGACTCGCCTGAAACGAACCGCTCGG AGAAGGTATACACGTCGCAAGAACCGAATATGTTA CTTACAAGAAATTTTTAGCAATGAGATGGCCAAA GTTGACGATTCTTTCTTTCACCGTTTGGAAGAGTC CTTCCTTGTCGAAGAGGACAAGAAACATGAACGG CACCCCATCTTTGGAAACATAGTAGATGAGGTGGC ATATCATGAAAAGTACCCAACGATTTATCACCTC AGAAAAAAGCTAGTTGACTCAACTGATAAAGCGGA CCTGAGGTTAATCTACTTGGCTCTTGCCCATATG ATAAAGTTCCGTGGGCACTTTCTCATTGAGGGTGA TCTAAATCCGGACAACTCGGATGTCGACAAACTG TTCATCCAGTTAGTACAAACCTATAATCAGTTGTT TGAAGAGAACCCTATAAATGCAAGTGGCGTGGAT GCGAAGGCTATTCTTAGCGCCCGCCTCTCTAAATC CCGACGGCTAGAAAACCTGATCGCACAATTACCC GGAGAGAAGAAAAATGGGTTGTTCGGTAACCTTAT AGCGCTCTCACTAGGCCTGACACCAAATTTTAAG TCGAACTTCGACTTAGCTGAAGATGCCAAATTGCA GCTTAGTAAGGACACGTACGATGACGATCTCGAC AATCTACTGGCACAAATTGGAGATCAGTATGCGGA CTTATTTTTGGCTGCCAAAAACCTTAGCGATGCA ATCCTCCTATCTGACATACTGAGAGTTAATACTGA GATTACCAAGGCGCCGTTATCCGCTTCAATGATC AAAAGGTACGATGAACATCACCAAGACTTGACACT TCTCAAGGCCCTAGTCCGTCAGCAACTGCCTGAG AAATATAAGGAAATATTCTTTGATCAGTCGAAAAA CGGGTACGCAGGTTATATTGACGGCGGAGCGAGT CAAGAGGAATTCTACAAGTTTATCAAACCCATATT AGAGAAGATGGATGGGACGGAAGAGTTGCTTGTA AAACTCAATCGCGAAGATCTACTGCGAAAGCAGCG GACTTTCGACAACGGTAGCATTCCACATCAAATC CACTTAGGCGAATTGCATGCTATACTTAGAAGGCA GGAGGATTTTTATCCGTTCCTCAAAGACAATCGT GAAAAGATTGAGAAAATCCTAACCTTTCGCATACC TTACTATGTGGGACCCCTGGCCCGAGGGAACTCT CGGTTCGCATGGATGACAAGAAAGTCCGAAGAAAC GATTACTCCCTGGAATTTTGAGGAAGTTGTCGAT AAAGGTGCGTGAGCTCAATCGTTCATCGAGAGGAT GACGgccTTTGACAAGAATTTACCGAACGAAAAA GTATTGCCTAAGCACAGTTTACTTTACGAGTATTT CACAGTGTACAATGAACTCACGAAAGTTAAGTAT GTCACTGAGGGCATGCGTAAATCCGCCTTTCTAAG CGGAGAACAGAAGAAAGCAATAGTAGATCTGTTA TTCAAGACCAACCGCAAAGTGACAGTTAAGCAATT GAAAGAGGACTACTTTAAGAAAATTGAATGCTTC GATTCTGTCGAGATCTCCGGGGTAGAAGATCGATT TAATGCGTCACTTGGTACGTATCATGACCTCCTA AAGATAATTAAAGATAAGGACTTCCTGGATAACGA AGAGAATGAAGATATCTTAGAAGATATAGTGTTG ACTCTTACCCTCTTTGAAGATCGGGAAATGATTGA GGAAAGACTAAAAACATACGCTCACCTGTTCGAC GATAAGGTTATGAAACAGTTAAAGAGGCGTCGCTA TACGGGCTGGGGAgccTTGTCGCGGAAACTTATC AACGGGATAAGAGACAAGCAAAGTGGTAAAACTAT TCTCGATTTTCTAAAGAGCGACGGCTTCGCCAAT AGGAACTTTATGgccCTGATCCATGATGACTCTTT AACCTTCAAAGAGGATATACAAAAGGCACAGGTT TCCGGACAAGGGGACTCATTGCACGAACATATTGC GAATCTTGCTGGTTCGCCAGCCATCAAAAAGGGC ATACTCCAGACAGTCAAAGTAGTGGATGAGCTAGT TAAGGTCATGGGACGTCACAAACCGGAAAACATT GTAATCGAGATGGCACGCGAAAATCAAACGACTCA GAAGGGGCAAAAAAACAGTCGAGAGCGGATGAAG AGAATAGAAGAGGGTATTAAAGAACTGGGCAGCCA GATCTTAAAGGAGCATCCTGTGGAAAATACCCAA TTGCAGAACGAGAAACTTTACCTCTATTACCTACA AAATGGAAGGGACATGTATGTTGATCAGGAACTG GACATAAACCGTTTATCTGATTACGACGTCGATCA CATTGTACCCCAATCCTTTTTGAAGGACGATTCA ATCGACAATAAAGTGCTTACACGCTCGGATAAGAA CCGAGGGAAAAGTGACAATGTTCCAAGCGAGGAA GTCGTAAAGAAAATGAAGAACTATTGGCGGCAGCT CCTAAATGCGAAACTGATAACGCAAAGAAAGTTC GATAACTTAACTAAAGCTGAGAGGGGTGGCTTGTC TGAACTTGACAAGGCCGGATTTATTAAACGTCAG CTCGTGGAAACCCGCgccATCACAAAGCATGTTGC GCAGATACTAGATTCCCGAATGAATACGAAATAC GACGAGAACGATAAGCTGATTCGGGAAGTCAAAGT AATCACTTTAAAGTCAAAATTGGTGTCGGACTTC AGAAAGGATTTTCAATTCTATAAAGTTAGGGAGAT AAATAACTACCACCATGCGCACGACGCTTATCTT AATGCCGTCGTAGGGACCGCACTCATTAAGAAATA CCCGAAGCTAGAAAGTGAGTTTGTGTATGGTGAT TACAAAGTTTATGACGTCCGTAAGATGATCGCGAA AAGCGAACAGGAGATAGGCAAGGCTACAGCCAAA TACTTCTTTTATTCTAACATTATGAATTTCTTTAA GACGGAAATCACTCTGGCAAACGGAGAGATACGC AAACGACCTTTAATTGAAACCAATGGGGAGACAGG TGAAATCGTATGGGATAAGGGCCGGGACTTCGCG ACGGTGAGAAAAGTTTTGTCCATGCCCCTAGTCAA CATAGTAAAGAAAACTGAGGTGCAGACCGGAGGG TTTTCAAAGGAATCGATTCTTCCAAAAAGGAATAG TGATAAGCTCATCGCTCGTAAAAAGGACTGGGAC CCGAAAAAGTACGGTGGCTTCgtgAGCCCTACAGT TGCCTATTCTGTCCTAGTAGTGGCAAAAGTTGAG AAGGGAAAATCGAAGAAACTGAAGTCAGTCAAAGA ATTATTGGGGATAACGATTATGGAGCGCTCGTCT TTTGAAAAGAACCCCATCGACTTCCTTGAGGCGAA AGGTTACAAGGAAGTAAAAAAGGATCTCATAATT AAACTACCAAAGTATAGTCTGTTTGAGTTAGAAAA TGGCCGAAAACGGATGTTGGCTAGCGCCGGAGAG CTTCAAAAGGGGAACGAACTCGCACTACCGTCTAA ATACGTGAATTTCCTGTATTTAGCGTCCCATTAC GAGAAGTTGAAAGGTTCACCTGAAGATAACGAACA GAAGCAACTTTTTGTTGAGCAGCACAAACATTAT CTCGACGAAATCATAGAGCAAATTTCGGAATTCAG TAAGAGAGTCATCCTAGCTGATGCCAATCTGGAC AAAGTATTAAGCGCATACAACAAGCACAGGGATAA ACCCATACGTGAGCAGGCGGAAAATATTATCCAT TTGTTTACTCTTACCAACCTCGGCGCTCCAGCCGC ATTCAAGTATTTTGACACAACGATAGATCGCAAA cagTACaqaTCTACCAAGGAGGTGCTAGACGCGAC ACTGATTCACCAATCCATCACGGGATTATATGAA ACTCGGATAGATTTGTCACAGCTTGGGGGTGACGG ATCCCCCAAGAAGAAGAGGAAAGTCTCGAGCGAC TACAAAGACCATGACGGTGATTATAAAGATCATGA CATCGATTACAAGGATGACGATGACAAGTGA

SEQ ID NO:277—BPK2797: CMV-T7-humanSpCas9-VRQR(D1135V, G1218R, R1335Q, T1337R)-NLS-3xFLAG

Human codon optimized S. pyogenes Cas9 in normal font, modified codons in lower case, NLS double underlined, 3xFLAG tag in bold:

ATGGATAAAAAGTATTCTATTGGTTTAGACATCGG CACTAATTCCGTTGGATGGGCTGTCATAACCGAT GAATACAAAGTACCTTCAAAGAAATTTAAGGTGTT GGGGAACACAGACCGTCATTCGATTAAAAAGAAT CTTATCGGTGCCCTCCTATTCGATAGTGGCGAAAC GGCAGAGGCGACTCGCCTGAAACGAACCGCTCGG AGAAGGTATACACGTCGCAAGAACCGAATATGTTA CTTACAAGAAATTTTTAGCAATGAGATGGCCAAA GTTGACGATTCTTTCTTTCACCGTTTGGAAGAGTC CTTCCTTGTCGAAGAGGACAAGAAACATGAACGG CACCCCATCTTTGGAAACATAGTAGATGAGGTGGC ATATCATGAAAAGTACCCAACGATTTATCACCTC AGAAAAAAGCTAGTTGACTCAACTGATAAAGCGGA CCTGAGGTTAATCTACTTGGCTCTTGCCCATATG ATAAAGTTCCGTGGGCACTTTCTCATTGAGGGTGA TCTAAATCCGGACAACTCGGATGTCGACAAACTG TTCATCCAGTTAGTACAAACCTATAATCAGTTGTT TGAAGAGAACCCTATAAATGCAAGTGGCGTGGAT GCGAAGGCTATTCTTAGCGCCCGCCTCTCTAAATC CCGACGGCTAGAAAACCTGATCGCACAATTACCC GGAGAGAAGAAAAATGGGTTGTTCGGTAACCTTAT AGCGCTCTCACTAGGCCTGACACCAAATTTTAAG TCGAACTTCGACTTAGCTGAAGATGCCAAATTGCA GCTTAGTAAGGACACGTACGATGACGATCTCGAC AATCTACTGGCACAAATTGGAGATCAGTATGCGGA CTTATTTTTGGCTGCCAAAAACCTTAGCGATGCA ATCCTCCTATCTGACATACTGAGAGTTAATACTGA GATTACCAAGGCGCCGTTATCCGCTTCAATGATC AAAAGGTACGATGAACATCACCAAGACTTGACACT TCTCAAGGCCCTAGTCCGTCAGCAACTGCCTGAG AAATATAAGGAAATATTCTTTGATCAGTCGAAAAA CGGGTACGCAGGTTATATTGACGGCGGAGCGAGT CAAGAGGAATTCTACAAGTTTATCAAACCCATATT AGAGAAGATGGATGGGACGGAAGAGTTGCTTGTA AAACTCAATCGCGAAGATCTACTGCGAAAGCAGCG GACTTTCGACAACGGTAGCATTCCACATCAAATC CACTTAGGCGAATTGCATGCTATACTTAGAAGGCA GGAGGATTTTTATCCGTTCCTCAAAGACAATCGT GAAAACATTGAGAAAATCCTAACCTTTCGCATACC TTACTATGTGGGACCCCTGGCCCGAGGGAACTCT CGGTTCGCATGGATGACAAGAAAGTCCGAAGAAAC GATTACTCCATGGAATTTTGAGGAAGTTGTCGAT AAAGGTGCGTCAGCTCAATCGTTCATCGAGAGGAT GACCAACTTTGACAAGAATTTACCGAACGAAAAA GTATTGCCTAAGCACAGTTTACTTTACGAGTATTT CACAGTGTACAATGAACTCACGAAAGTTAAGTAT GTCACTGAGGGCATGCGTAAACCCGCCTTTCTAAG CGGAGAACAGAAGAAAGCAATAGTAGATCTGTTA TTCAAGACCAACCGCAAAGTGACAGTTAAGCAATT GAAAGAGGACTACTTTAAGAAAATTGAATGCTTC GATTCTGTCGAGATCTCCGGGGTAGAAGATCGATT TAATGCGTCACTTGGTACGTATCATGACCTCCTA AAGATAATTAAAGATAAGGACTTCCTGGATAACGA AGAGAATGAAGATATCTTAGAAGATATAGTGTTG ACTCTTACCCTCTTTGAAGATCGGGAAATGATTGA GGAAAGACTAAAAACATACGCTCACCTGTTCGAC GATAAGGTTATGAAACAGTTAAAGAGGCGTCGCTA TACGGGCTGGGGACGATTGTCGCGGAAACTTATC AACGGGATAAGAGACAAGCAAAGTGGTAAAACTAT TCTCGATTTTCTAAAGAGCGACGGCTTCGCCAAT AGGAACTTTATGCAGCTGATCCATGATGACTCTTT AACCTTCAAAGAGGATATACAAAAGGCACAGGTT TCCGGACAAGGGGACTCATTGCACGAACATATTGC GAATCTTGCTGGTTCGCCAGCCATCAAAAAGGGC ATACTCCAGACAGTCAAAGTAGTGGATGAGCTAGT TAAGGTCATGGGACGTCACAAACCGGAAAACATT GTAATCGAGATGGCACGCGAAAATCAAACGACTCA GAAGGGGCAAAAAAACAGTCGAGAGCGGATGAAG AGAATAGAAGAGGGTATTAAAGAACTGGGCAGCCA GATCTTAAAGGAGCATCCTGTGGAAAATACCCAA TTGCAGAACGAGAAACTTTACCTCTATTACCTACA AAATGGAAGGGACATGTATGTTGATCAGGAACTG GACATAAACCGTTTATCTGATTACGACGTCGATCA CATTGTACCCCAATCCTTTTTGAAGGACGATTCA ATCGACAATAAAGTGCTTACACGCTCGGATAAGAA CCGAGGGAAAAGTGACAATGTTCCAAGCGAGGAA GTCGTAAAGAAAATGAAGAACTATTGGCGGCAGCT CCTAAATGCGAAACTGATAACGCAAAGAAAGTTC GATAACTTAACTAAAGCTGAGAGGGGTGGCTTGTC TGAACTTGACAAGGCCGGATTTATTAAACGTCAG CTCGTGGAAACCCGCCAAATCACAAAGCATGTTGC ACAGATACTAGATTCCCGAATGAATACGAAATAC GACGAGAACGATAAGCTGATTCGGGAAGTCAAAGT AATCACTTTAAAGTCAAAATTGGTGTCGGACTTC AGAAAGGATTTTCAATTCTATAAAGTTAGGGAGAT AAATAACTACCACCATGCGCACGACGCTTATCTT AATGCCGTCGTAGGGACCGCACTCATTAAGAAATA CCCGAAGCTAGAAAGTGAGTTTGTGTATGGTGAT TACAAAGTTTATGACGTCCGTAAGATGATCGCGAA AAGCGAACAGGAGATAGGCAAGGCTACAGCCAAA TACTTCTTTTATTCTAACATTATGAATTTCTTTAA GACGGAAATCACTCTGGCAAACGGAGAGATACGC AAACGACCTTTAATTGAAACCAATGGGGAGACAGG TGAAATCGTATGGGATAAGGGCCGGGACTTCGCG ACGGTGAGAAAAGTTTTGTCCATGCCCCAAGTCAA CATAGTAAAGAAAACTGAGGTGCAGACCGGAGGG TTTTCAAAGGAATCGATTCTTCCAAAAAGGAATAG TGATAAGCTCATCGCTCGTAAAAAGGACTGGGAC CCGAAAAAGTACGGTGGCTTCGTGAGCCCTACAGT TGCCTATTCTGTCCTAGTAGTGGCAAAAGTTGAG AAGGGAAAATCCAAGAAACTGAAGTCAGTCAAAGA ATTATTGGGGATAACGATTATGGAGCGCTCGTCT TTTGAAAAGAACCCCATCGACTTCCTTGAGGCGAA AGGTTACAAGGAAGTAAAAAAGGATCTCATAATT AAACTACCAAAGTATAGTCTGTTTGAGTTAGAAAA TGGCCGAAAACGGATGTTGGCTAGCGCCAGAGAG CTTCAAAAGGGGAACGAACTCGCACTACCGTCTAA ATACGTGAATTTCCTGTATTTAGCGTCCCATTAC GAGAAGTTGAAAGGTTCACCTGAAGATAACGAACA GAAGCAACTTTTTGTTGAGCAGCACAAACATTAT CTCGACGAAATCATAGAGGAAATTTCGGAATTCAG TAAGAGAGTCATCCTAGCTGATGCCAATCTGGAC AAAGTAATAAGCGCATACAACAAGCACAGGGATAA ACCCATACGTGAGCAGGCGGAAAATATTATCCAT TTGTTTACTCTTACCAACCTCGGCGCTCCAGCCGC ATTCAAGTATTTTGACACAACGATAGATCGCAAA CAGTACAGATCTACCAAGGAGGTGCTAGACGCGAC ACTGATTCACCAATCCATCACGGGATTATATGAA ACTCGGATAGATTTGTCACAGCTTGGGGGTGACGG ATCCCCCAAGAAGAAGAGGAAAGTCTCGAGCGAC TACAAAGACCATGACGGTGATTATAAAGATCATGA CATCGATTACAAGGATGACGATGACAAGTGA

SEQ ID NO:278—MSP2443: CMV-T7-humanSpCas9-VRQR-HF1(N497A, R661A, Q695A, Q926A, D1135V, G1218, R1335Q, T1337R)-NLS-3xFLAG

Human codon optimized S. pyogenes Cas9 in normal font, modified codons in lower case, NLS double underlined, 3xFLAG taq in bold:

ATGGATAAAAAGTATTCTATTGGTTTAGACATCGG CACTAATTCCGTTGGATGGGCTGTCATAACCGAT GAATACAAAGTACCTTCAAAGAAATTTAAGGTGTT GGGGAACACAGACCGTCATTCGATTAAAAAGAAT CTTATCGGTGCCCTCCTATTCGATAGTGGCGAAAC GGCAGAGGCGACTCGCCTGAAACGAACCGCTCGG AGAAGGTATACACGTCGCAAGAACCGAATATGTTA CTTACAAGAAATTTTTAGCAATGAGATGGCCAAA GTTGACGATTCTTTCTTTCACCGTTTGGAAGAGTC CTTCCTTGTCGAAGAGGACAAGAAACATGAACGG CACCCCATCTTTGGAAACATAGTAGATGAGGTGGC ATATCATGAAAAGTACCCAACGATTTATCACCTC AGAAAAAAGCTAGTTGACTCAACTGATAAAGCGGA CCTGAGGTTAATCTACTTGGCTCTTGCCCATATG ATAAAGTTCCGTGGGCACTTTCTCATTGAGGGTGA TCTAAATCCGGACAACTCGGATGTCGACAAACTG TTCATCCAGTTAGTACAAACCTATAATCAGTTGTT TGAAGAGAACCCTATAAATGCAAGTGGCGTGGAT GCGAAGGCTATTCTTAGCGCCCGCCTCTCTAAATC CCGACGGCTAGAAAACCTGATCGCACAATTAGCC GGAGAGAAGAAAAATGGGTTGTTCGGTAACCTTAT AGCGCTCTCACTAGGCCTGACACCAAATTTTAAG TCGAACTTCGACTTAGCTGAAGATGCCAAATTGCA GCTTAGTAAGGACACGTACGATGACGATCTCGAC AATCTACTGGCACAAATTGGAGATCAGTATGCGGA CTTATTTTTGGCTGCCAAAAACCTTAGCGATGCA ATCCTCCTATCTGACATACTGAGAGTTAATACTGA GATTACCAAGGCGCCGTTATCCGCTTCAATGATC AAAAGGTACGATGAACATCACCAAGACTTGACACT TCTCAAGGCCCTAGTCCGTCAGCAACTGCCTGAG AAATATAAGGAAATATTCTTTGATCAGTCGAAAAA CGGGTACGCAGGTTATATTGACGGCGGAGCGAGT CAAGAGGAATTCTACAAGTTTATCAAACCCATATT AGAGAAGATGGATGGGACGGAAGAGTTGCTTGTA AAACTCAATCGCGAAGATCTACTGCGAAAGCAGCG GACTTTCGACAACGGTAGCATTCCACATCAAATC CACTTAGGCGAATTGCATGCTATACTTAGAAGGCA GGAGGATTTTTATCCGTTCCTCAAAGACAATCGT GAAAAGATTGAGAAAATCCTAACCTTTCGCATACC TTACTATGTGGGACCCCTGGCCCGAGGGAACTCT CGGTTCGCATGGATGACAAGAAAGTCCGAAGAAAC GATTACTCCCTGGAATTTTGAGGAAGTTGTCGAT AAAGGTGCGTCAGCTCAATCGTTCATCGAGAGGAT GACCGCCTTTGACAAGAATTTACCGAACGAAAAA GTATTGCCTAAGCACAGTTTACTTTACGAGTATTT CACAGTGTACAATGAACTCACGAAAGTTAAGTAT GTCACTGAGGGCATGCGTAAACCCGCCTTTCTAAG CGGAGAACAGAAGAAAGCAATAGTAGATCTGTTA TTCAAGACCAACCGCAAAGTGACAGTTAAGCAATT GAAAGAGGACTACTTTAAGAAAATTGAATGCTTC GATTCTGTCGAGATCTCCGGGGTAGAAGATCGATT TAATGCGTCACTTGGTACGTATCATGACCTCCTA AAGATAATTAAAGATAAGGACTTCCTGGATAACGA AGAGAATGAAGATATCTTAGAAGATATAGTGTTG ACTCTTACCCTCTTTGAAGATCGGGAAATGATTGA GGAAAGACTAAAAACATACGCTCACCTGTTCGAC CATAAGGTTATGAAACAGTTAAAGAGGCGTCGCTA TACGGGCTGGGGAGCCTTGTCGCGGAAACTTATC AACGGGATAAGAGACAAGCAAAGTGGTAAAACTAT TCTCGATTTTCTAAAGAGCGACGGCTTCGCCAAT AGGAACTTTATGGCCCTGATCCATGATGACTCTTT AACCTTCAAAGAGGATATACAAAAGGCACAGGTT TCCGGACAAGGGGACTCATTGCACGAACATATTGC GAATCTTGCTGGTTCGCCAGCCATCAAAAAGGGC ATACTCCAGACAGTCAAAGTAGTGGATGAGCTAGT TAAGGTCATGGGACGTCACAAACCGGAAAACATT GTAATCGAGATGGCACGCGAAAATCAAACGACTCA GAAGGGGCAAAAAAACAGTCGAGAGCGGATGAAG AGAATAGAAGAGGGTATTAAAGAACTGGGCAGCGA GATCTTAAAGGAGCATCCTGTGGAAAATACCCAA TTGCAGAACGAGAAACTTTACCTCTATTACCTACA AAATGGAAGGGACATGTATGTTGATCAGGAACTG GACATAAACCGTTTATCTGATTACGACGTCGATCA CATTGTACCCCAATCCTTTTTGAAGGACGATTCA ATCGACAATAAAGTGCTTACACGCTCGGATAAGAA CCGAGGGAAAAGTGACAATGTTCCAAGCGAGGAA GTCGTAAAGAAAATGAAGAACTATTGGCGGCAGCT CCTAAATGCGAAACTGATAACGCAAAGAAAGTTC GATAACTTAACTAAAGCTGAGAGGGGTGGCTTGTC TGAACTTGACAAGGCCGGATTTATTAAACGTCAG CTCGTGGAAACCCGCGCCATCACAAAGCATGTTGC GCAGATACTAGATTCCCGAATGAATACGAAATAC GACGAGAACGATAAGCTGATTCGGGAAGTCAAAGT AATCACTTTAAAGTCAAAATTGGTGTCGGACTTC AGAAAGGATTTTCAATTCTATAAAGTTAGGGAGAT AAATAACTACCACCATGCGCACGACGCTTATCTT AATGCCGTCGTAGGGACCGCACTCATTAAGAAATA CCCGAAGCTAGAAAGTGAGTTTGTGTATGGTGAT TACAAAGTTTATGACGTCCGTAAGATGATCGCGAA AAGCGAACAGGAGATAGGCAAGGCTACAGCCAAA TACTTCTTTTATTCTAACATTATGAATTTCTTTAA GACGGAAATCACTCTGGCAAACGGAGAGATACGC AAACGACCTTTAATTGAAACCAATGGGGAGACAGG TGAAATCGTATGGGATAAGGGCCGGGACTTCGCG TTTTCAAAGGAATCGATTCTTCCAAAAAGGAATAG TGATAAGCTCATCGCTCGTAAAAAGGACTGGGAC CCGAAAAAGTACGGTGGCTTCgtgAGCCCTACAGT TGCCTATTCTGTCCTAGTAGTGGCAAAAGTTGAG AAGGGAAAATCCAAGAAACTGAAGTCAGTCAAAGA ATTATTGGGGATAACGATTATGGAGCGCTCGTCT TTTGAAAAGAACCCCATCGACTTCCTTGAGGCGAA AGGTTACAAGGAAGTAAAAAAGGATCTCATAATT AAACTACCAAAGTATAGTCTGTTTGAGTTAGAAAA TGGCCGAAAACGGATGTTGGCTAGCGCCagaGAG CTTCAAAAGGGGAACGAACTCGCACTACCGTCTAA ATACGTGAATTTCCTGTATTTAGCGTCCCATTAC GAGAAGTTGAAAGGTTCACCTGAAGATAACGAACA GAAGCAACTTTTTGTTGAGCAGCACAAACATTAT CTCGACGAAATCATAGAGCAAATTTCGGAATTCAG TAAGAGAGTCATCCTAGCTGATGCCAATCTGGAC AAAGTATTAAGCGCATACAACAAGCACAGGGATAA ACCCATACGTGAGCAGGCGGAAAATATTATCCAT TTGTTTACTCTTACCAACCTCGGCGCTCCAGCCGC ATTCAAGTATTTTGACACAACGATAGATCGCAAA cagTACagaTCTACCAAGGAGGTGCTAGACGCGAC ACTGATTCACCAATCCATCACGGGATTATATGAA ACTCGGATAGATTTGTCACAGCTTGGGGGTGACGG ATCCCCCAAGAAGAAGAGGAAAGTCTCGAGCGAC TACAAAGACCATGACGGTGATTATAAAGATCATGA CATCGATTACAAGGATGACGATGACAAGTGA

SEQ ID NO:279—BPK1520: U6-BsmBIcassette-Sp-sgRNA U6 promoter in normal font, BsmBI sites italicized, S. pyogenes sgRNA in lower case, U6 terminator double underlined:

TGTACAAAAAAGCAGGCTTTAAAGGAACCAATTCAGTCGACTGGATCCGG TACCAAGGTCGGGCAGGAAGAGGGCCTATTTCCCATGATTCCTTCATATT TGCATATACGATACAAGGCTGTTAGAGAGATAATTAGAATTAATTTGACT GTAAACACAAAGATATTAGTACAAAATACGTGACGTAGAAAGTAATAATT TCTTGGGTAGTTTGCAGTTTTAAAATTATGTTTTAAAATGGACTATCATA TGCTTACCGTAACTTGAAAGTATTTCGATTTCTTGGCTTTATATATCTTG TGGAAAGGACGAAACACCG GAGACG ATTAATG CGTCTC Cgttttagagct agaaatagcaagttaaaataaggctagtccgttatcaacttgaaaaagtg gcaccgagtcggtgcttttttt

OTHER EMBODIMENTS

It is to be understood that while the invention has been described in conjunction with the detailed description thereof, the foregoing description is intended to illustrate and not limit the scope of the invention, which is defined by the scope of the appended claims. Other aspects, advantages, and modifications are within the scope of the following claims. 

What is claimed is:
 1. An isolated Staphylococcus aureus Cas9 (SaCas9) protein that is at least 95% identical to SEQ ID NO: 2, with mutations at one, two, three, four, five, six, or more of the following positions: Y211, Y212, W229, Y230, R245, T392, N419, Y651, or R654.
 2. The isolated protein of claim 1, comprising one or more of the following mutations: Y211A, Y212A, W229, Y230A, R245A, T392A, N419A, Y651A, and/or R654A.
 3. The isolated protein of claim 1, comprising mutations at N419 and/or R654, and optionally one, two, three, four or more of the additional mutations at Y211, Y212, W229, Y230, R245, T392, and Y651.
 4. The isolated protein of claim 3, comprising mutations at N419A/R654A, Y211A/R654A, Y211A/Y212A, Y211A/Y230A, Y211A/R245A, Y212A/Y230A, Y212A/R245A, Y230A/R245A, W229A/R654A, Y211A/Y212A/Y230A, Y211A/Y212A/R245A, Y211A/Y212A/Y651A, Y211A/Y230A/R245A, Y211A/Y230A/Y651A, Y211A/R245A/Y651A, Y211A/R245A/R654A, Y211A/R245A/N419A, Y211A/N419A/R654A, Y212A/Y230A/R245A, Y212A/Y230A/Y651A, Y212A/R245A/Y651A, Y230A/R245A/Y651A, R245A/N419A/R654A, T392A/N419A/R654A, R245A/T392A/N419A/R654A, Y211A/R245A/N419A/R654A, W229A/R245A/N419A/R654A, Y211A/R245A/T392A/N419A/R654A, or Y211A/W229A/R245A/N419A/R654A.
 5. The isolated protein of claim 1, further comprising mutations at N44; R45; R51; R55; K57; R59; R60; R61; H111; K114; R116; V164; R165; N169; R208; R209; T238; Y239; K248; Y256; R314; N394; Q414; L446; Q488A; N492A; Q495A; R497A; N498A; R499; Q500; K518; K523; K525; H557; R561; K572; R634; G655; N658; S662; N667; R686; K692; R694; H700; K751; D786; T787; L788Y789; S790; R792; N804; Y868; K870; K878; K879; K881; T882; K886; Y897N888; A889; R901; K906; L909; N985; N986; R991; and/or R1015.
 6. The isolated protein of claim 1, further comprising one or more of the following mutations: E782K; K929R; N968K; R1015H; E782K/N968K/R1015H (KKH variant); E782K/K929R/R1015H (KRH variant); or E782K/K929R/N968K/R1015H (KRLKH variant).
 7. The isolated protein of claim 1, further comprising mutations that decrease nuclease activity said mutations at H557 or N580 and at D10, E477, D556, H701, or D704.
 8. The isolated protein of claim 7, wherein the mutations at D10 are D10A or D10N, the mutation at D556 is D556A, the mutations at H557 are H557A, H557N, or H557Y and the mutation at N580 is N580A.
 9. The isolated protein of claim 1, wherein the SaCas9 protein is fused to one or more of a nuclear localization sequence, cell penetrating peptide sequence, and/or affinity tag.
 10. A fusion protein comprising the isolated protein of claim 1, fused to a heterologous functional domain, with an optional intervening linker, wherein the linker does not interfere with activity of the fusion protein.
 11. The fusion protein of claim 10, wherein the heterologous functional domain is a transcriptional activation domain.
 12. The fusion protein of claim 11, wherein the transcriptional activation domain is from VP64 or NF-KB p65.
 13. The fusion protein of claim 10, wherein the heterologous functional domain is a transcriptional silencer or transcriptional repression domain.
 14. The fusion protein of claim 13, wherein the transcriptional repression domain is a Krueppel-associated box (KRAB) domain, ERF repressor domain (ERD), or mSin3A interaction domain (SID).
 15. The fusion protein of claim 13, wherein the transcriptional silencer is Heterochromatin Protein 1 (HP1).
 16. The fusion protein of claim 15, wherein the HP1 is HP1α or HP1β.
 17. The fusion protein of claim 10, wherein the heterologous functional domain is an enzyme that modifies the methylation state of DNA.
 18. The fusion protein of claim 17, wherein the enzyme that modifies the methylation state of DNA is a DNA methyltransferase (DNMT) or a TET protein.
 19. The fusion protein of claim 18, wherein the TET protein is TET1.
 20. The fusion protein of claim 10, wherein the heterologous functional domain is an enzyme that modifies a histone subunit.
 21. The fusion protein of claim 20, wherein the enzyme that modifies a histone subunit is a histone acetyltransferase (HAT), histone deacetylase (HDAC), histone methyltransferase (HMT), or histone demethylase.
 22. The fusion protein of claim 10, wherein the heterologous functional domain is a biological tether.
 23. The fusion protein of claim 22, wherein the biological tether is MS2, Csy4 or lambda N protein.
 24. The fusion protein of claim 10, wherein the heterologous functional domain is FokI.
 25. An isolated nucleic acid encoding the protein of claim
 1. 26. A vector comprising the isolated nucleic acid of claim 25, optionally operably linked to one or more regulatory domains.
 27. A host cell comprising the nucleic acid of claim
 25. 28. A method of altering the genome or epigenome of a cell, the method comprising expressing in the cell or contacting the cell with the isolated protein of claim 1 and a guide RNA having a region complementary to a selected portion of the genome of the cell.
 29. A method of altering the genome or epigenome of a cell, the method comprising expressing in the cell or contacting the cell with the isolated fusion protein of claim 10 and a guide RNA having a region complementary to a selected portion of the genome of the cell.
 30. A method of altering a double stranded DNA (dsDNA) molecule, the method comprising contacting the dsDNA molecule with the isolated protein of claim 1, and a guide RNA having a region complementary to a selected portion of the dsDNA molecule.
 31. The method of claim 30, wherein the dsDNA molecule is in vitro.
 32. A method of altering a double stranded DNA D (dsDNA) molecule, the method comprising contacting the dsDNA molecule with the fusion protein of claim 10, and a guide RNA having a region complementary to a selected portion of the dsDNA molecule. 